Ehrlichial invasin for immuniztion, diagnosis, and cell delivery

ABSTRACT

Disclosed are vaccines containing one or more immunogenic polypeptides derived from an EtpE protein from an  Ehrlichia  sp. or nucleic acid encoding these polypeptides. Also disclosed is a method for vaccinating a subject against  Ehrlichia  sp. that involves administering to the subject a composition comprising any of the disclosed vaccines. Also disclosed is a method for diagnosing and/or monitoring the treatment of Ehrlichiosis in a subject that comprising assaying a biological sample (e.g., blood, serum, or plasma sample) from the subject for the presence of an antibody that specifically binds an EtpE polypeptide. Also disclosed are methods for delivering a therapeutic or diagnostic agent to a cell in a subject that involves conjugating the agent, or a delivery vehicle comprising the agent, to polypeptide containing the C-terminal domain of an EtpE protein.

CROSS-REFERENCE TO RELATED APPLICATIONS

This application is a divisional of co-pending application Ser. No. 15/362,137, filed Nov. 28, 2016, which is a divisional of Ser. No. 14/649,138 (now U.S. Pat. No. 9,526,772), filed Jun. 2, 2015, which is a National Stage Application of PCT/US2013/072850, filed Dec. 12, 2013, which claims benefit of U.S. Provisional Application No. 61/732,491, filed Dec. 3, 2012, and U.S. Provisional Application No. 61/810,039, filed Apr. 9, 2013, all of which are hereby incorporated herein by reference in their entirety.

STATEMENT REGARDING FEDERALLY SPONSORED RESEARCH OR DEVELOPMENT

This invention was made with Government Support under Grant No. R01AI30010 and Grant No. R01AI047885 awarded by the National Institutes of Health. The Government has certain rights in the invention.

REFERENCE TO SEQUENCE LISTING

The Sequence Listing submitted filed Jan. 11, 2019, as a text file named “10336-055US3 2018_01_11 SEQUENCE LISTING.TXT”, created on Jan. 11, 2019, and having a size of 90 KB, is hereby incorporated by reference pursuant to 37 C.F.R. § 1.52(e)(5).

BACKGROUND

Ehrlichia chaffeensis causes human monocytic ehrlichiosis (HME), an emerging tick-borne zoonosis. From the site of infected tick bite on human skin, E. chaffeensis infects monocytes and spreads via the bloodstream to various tissues, causing a systemic febrile disease. HME is characterized by fever, headache, myalgia, thrombocytopenia, leucopenia, and elevated liver-enzyme levels, but complications such as pulmonary insufficiency, renal failure, encephalopathy, and disseminated intravascular coagulation can cause death [Paddock C D, et al. (2003) Clin Microbiol Rev 16: 37-64]. Early diagnosis and the proper treatment with doxycycline are critical to prevent complications. The disease is of particular threat to the immunocompromised and the elderly people [Paddock C D, et al. (2003) Clin Microbiol Rev 16: 37-64].

E. chaffeensis is a small obligatory intracellular bacterium. It belongs to the family Anaplasmataceae in the order Rickettsiales that includes many understudied pathogens of veterinary and public health importance [Rikihisa Y (2010) Nat Rev Microbiol 8: 328-339]. By electron microscopy, E. chaffeensis is a polymorphic bacterium (0.2-2.0 μm in diameter), and can be morphologically categorized as small dense-cored cells (DCs) or large reticulate cells (RCs) [Popov V L, et al. (1995) J Med Microbiol 43: 411-421]. DCs are approximately 0.2-0.5 μm in diameter, which is close to the size of the elementary body of Chlamydia and larger viruses such as Vaccinia virus. By light microscopy, it is not possible to distinguish individual RCs and DCs, since E. chaffeensis aggregates inside eukaryotic host cells. The characteristic clump of intracellular E. chaffeensis organisms is termed as “morula” (mulberry in Latin) [Rikihisa Y (2010) Nat Rev Microbiol 8: 328-339]. However, when they are freshly isolated from host cells and dispersed, smaller bacteria (<0.5 μm) are more densely stained with basic dye than larger bacteria (>0.5 μm); therefore, they were defined as DCs and RCs, respectively [Zhang J Z, et al. (2007) Cell Microbiol 9: 610-618]. DCs are more resistant to strong sonication and more infectious than RCs [Cheng Z, et al. (2008) J Bacteriol 190: 2096-2105]. In cell culture, a biphasic developmental cycle has been reported: initially small infectious DCs bind to and internalize into host cells, which then develop into larger replicating RCs inside a membrane-lined compartment that resembles early endosomes. After replication in expanding inclusions, the mature RCs transform back into DCs prior to release from the host cells [Zhang J Z, et al. (2007) Cell Microbiol 9: 610-618; Cheng Z, et al. (2008) J Bacteriol 190: 2096-2105]. In patients' blood specimens, monocytes were primarily infected with E. chaffeensis, and hence, the disease was named as “monocytic ehrlichiosis” to distinguish it from “granulocytic ehrlichiosis” caused by infection with granulocyte-tropic Ehrlichia sp. [Paddock C D, et al. (2003) Clin Microbiol Rev 16: 37-64]. E. chaffeensis can replicate well in several mammalian cell lines including canine histiocytic leukemia (DH82), human acute leukemia (THP-1), human promyelocytic leukemia (HL-60), human embryonic kidney (HEK293), and monkey endothelial (RF/6A) cells [Mott J, et al. (1999) Infect Immun 67: 1368-1378; Liu H, et al. (2012) Cell Microbiol 14: 1037-1050; Miura K, et al. (2011) Infect Immun 79: 4947-4956].

Entry into the permissive eukaryotic host cells is essential for E. chaffeensis to sustain its life, since its small genome of 1.18 Mb lacks a large portion of metabolic genes that are required for free living [Dunning Hotopp J C, et al. (2006) PLoS Genet 2:e21]. E. chaffeensis also lacks LPS, peptidoglycan, lipoteichoic acid, and flagella that engage Toll-like or NOD-like receptors, or scavenger receptors [Rikihisa Y (2010) Nat Rev Microbiol 8: 328-339; Rikihisa Y (2010) Nat Rev Microbiol 8: 328-339]. E. chaffeensis entry and subsequent infection of THP-1 cells, but not binding are almost completely inhibited by monodansylcadaverine (MDC), a transglutaminase inhibitor [Lin M, et al. (2002) Infect Immun 70: 889-898]. MDC is known to block Neorickettsia risticii (formerly Ehrlichia risticii) entry and infection of P388D1 cells, vesicular stomatitis virus uptake and receptor-mediated endocytosis of α2-macroglobulin by Swiss 3T3 mouse cells, but not the uptake of latex beads by P388D1 mouse macrophages [Levitzki A, et al. (1980) Proc Natl Acad Sci USA 77: 2706-2710; Messick J B, et al. (1993) Infect Immun 61: 3803-3810; Schlegel R, et al. (1982) Proc Natl Acad Sci USA 79:2291-2295]. E. chaffeensis entry into THP-1 cells, leading to productive infection, is dependent on the host-cell surface lipid rafts and glycosylphosphatidyl inositol (GPI)-anchored proteins [Lin M, Rikihisa Y (2003) Cell Microbiol 5: 809-820]. Furthermore, lipid raft-associated protein caveolin-1, but not clathrin localizes to the E. chaffeensis entry site [Lin M, Rikihisa Y (2003) Cell Microbiol 5: 809-820]. After entry, E. chaffeensis replicates in the membrane-bound compartment resembling an early endosome as it contains early endosome antigen 1 (EEA1), RabS, and transferrin receptor [Mott J, et al. (1999) Infect Immun 67: 1368-1378]. Several intracellular bacteria are known to enter host cells by using their specific surface protein collectively called as ‘invasin’ or ‘intemalin’ [Pizarro-Cerda J, et al. (2006) Cell 124: 715-727]. However, detailed mechanisms of E. chaffeensis entry were unknown; particularly regarding the involvement of any specific bacterial surface protein that can function as an invasin and its cognitive host-cell receptor [Rikihisa Y (2010) Nat Rev Microbiol 8: 328-339].

The importance of E. canis as a veterinary pathogen in conjunction with the recent identification of E. chaffeensis as the cause of an emerging tick-borne zoonosis has highlighted the need for improved diagnostics and vaccines for both veterinary and human ehrlichioses, and thus the need for identification of immunoreactive proteins.

SUMMARY

The comparative genome hybridization study of E. chaffeensis strains identified a protein (referred to herein as “entry triggering protein of Ehrlichia” or “EtpE”) with highly conserved N- and C-terminal segments flanking its strain-variable central region. As disclosed herein, EtpE, particularly its C-terminal conserved region (“EtpE-C”), is critical for Ehrlichia sp. binding, entry, and infection of several different host cell types. Immunization with rEtpE-C is also shown to protect mice against Ehrlichia sp. challenge. Further, antibodies to both the EtpE-C and the N-terminal region (“EtpE-N”) can be found in subjects infected with Ehrlichia sp. Importantly, the EtpE-N is highly conserved across Ehrlichia sp. Therefore, disclosed herein are vaccines, diagnostics, and cell delivery polypeptides and uses therefore that take advantage of these unique properties of EtpE.

In particular, a vaccine is disclosed that comprises one or more polypeptides representing the EtpE from an Ehrlichia sp. and a pharmaceutically acceptable adjuvant. For example, the one or more polypeptide can comprise the amino acid sequence SEQ ID NO:1 (EtpE from Ehrlichia chaffeensis str. Arkansas; Accession No. YP_507823.1), SEQ ID NO:3 (EtpE from Ehrlichia canis str. Jake; Accession No. AAZ68869.1), or SEQ ID NO:5 (EtpE from Ehrlichia ruminantium str. Welgevonden; Accession No. YP_180660.1). Additional sequences for EtpE orthologues include Ehrlichia HF strain (Ixodes ovatus Ehrlichia) (Accession No. ABM69271.1), Ehrlichia chaffeensis Sapulpa strain (Accession No. ZP 00544864.1 and ZP_00544886.1), and Ehrlichia ruminantium, Gardel strain (Accession No. YP_196760.1). EtpE homologues/orthologues from other Ehrlichia sp. can also be identified and used to improve species cross-reactivity.

In some embodiments, the vaccine contains an immunogenic fragment of an EtpE protein that is capable of eliciting an immune response against an Ehrlichia sp. Preferably, the immunogenic fragment comprises at least a portion of the conserved region (“EtpE-C”). For example, the one or more polypeptide can comprise the amino acid sequence SEQ ID NO:2 (residues 1656-1963 of SEQ ID NO:1), SEQ ID NO:4 (residues 1408-1510 of SEQ ID NO:3), SEQ ID NO:6 (residues 1410-1710 of SEQ ID NO:5), or a an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp.

The vaccine can alternatively contain an immunogenic variant of an EtpE protein, or fragment thereof, that is capable of eliciting an immune response against an Ehrlichia sp. For example, the vaccine can comprise one or more polypeptides having an amino acid sequence with at least 70% identity to an amino acid sequence selected from the group consisting of SEQ ID NO:1, SEQ ID NO:3, SEQ ID NO:5, or an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp. The vaccine can comprise one or more polypeptides having an amino acid sequence with at least 7% identity to SEQ ID NO:2, SEQ ID NO:4, SEQ ID NO:6, or a an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp.

The vaccine comprises polypeptides representing the EtpE from at least one Ehrlichia sp. However, to improve cross-reactivity, the vaccine can contain polypeptides representing the EtpE from at least 2, 3, 4, 5, 6, or more Ehrlichia sp. These polypeptides can be in a single amino acid sequence, such as fusion protein. The polypeptides can also be conjugated together on a single carrier molecule. For example, the polypeptides can be used in a multiple antigen peptide system (MAPS).

In some embodiments, the vaccine is capable of eliciting an immune response against any combination of Ehrlichia chaffeensis, Ehrlichia canis, and Ehrlichia ruminantium. The vaccine can also be capable of eliciting an immune response against other species, such as Ehrlichia muris, Ehrlichia ewingii, or a combination thereof. The EtpE homologue from these and other species and strains can be identified and used as immunogens as described herein.

Also disclosed is a recombinant vector that contains a nucleic acid sequence encoding any of the one or more immunogenic polypeptides disclosed herein, operatively linked to a heterologous promoter.

Also disclosed is a vaccine containing any of the disclosed recombinant vectors in a pharmaceutically acceptable vehicle, diluent or excipient. The vaccine can further contain a pharmaceutically acceptable adjuvant.

Also disclosed is a method for vaccinating a subject against Ehrlichia sp, that comprises administering to the subject a composition comprising any of the disclosed vaccines. The subject can be any mammal at risk for Ehrlichia sp. infection. In particular, the subject can be a human, canine, feline, bovine, ovine, or caprine subject. The method provides a protective immune response against at least one Ehrlichia sp. selected from the group consisting of Ehrlichia chaffeensis, Ehrlichia canis, and Ehrlichia ruminantium. However, in preferred embodiments, the vaccine elicits a protective immune response in the subject against at least 2, 3, 4, 5, 6, or more Ehrlichia sp.

Also disclosed is a method for diagnosing Ehrlichiosis in a subject that comprising assaying a biological sample (e.g., blood, serum, or plasma sample) from the subject for the presence of an antibody that specifically binds an EtpE polypeptide. In particular, assaying for antibodies that specifically bind an EtpE-N provides pan-diagnosis of Ehrlichia sp. infection since the N-terminal domain is highly conserved across species. Therefore, in some embodiments, the presence of the antibody is an indication that the subject has been infected with an Ehrlichia sp. selected from the group consisting of Ehrlichia chaffeensis, Ehrlichia canis, Ehrlichia ruminantium, or any combination thereof. Therefore, the method can involve assaying a biological sample from the subject for the presence of an antibody that specifically binds SEQ ID NO:7 (amino acid residues 29-708 of SEQ ID NO:1), SEQ ID NO:8 (amino acid residues 43-736 of SEQ ID NO:3), SEQ ID NO:9 (amino acid residues 39-730 of SEQ ID NO:5), or a conservative variant thereof having at least 70% identity to SEQ ID NO:7, SEQ ID NO:8, or SEQ ID NO:9, wherein the presence of the antibody is an indication that the subject has been infected with an Ehrlichia sp.

In some embodiments, the method provides a pan-diagnostic so that one test can be used for multiple species of Ehrlichia. However, in some embodiments, the method also diagnoses the specific Ehrlichia sp. In these embodiments, the EtpE-C polypeptide can be used to detect antibodies that selectively bind the C-terminal region of an EtpE from a specific species of Ehrlichia.

The disclosed methods can further comprise treating the subject for Ehrlichiosis if the antibody is detected. For example, the method can comprise treating the subject with an effective amount and duration of doxycycline if the antibody is detected. This should be done as early as possible, since at later stage of infection antibiotic became less effective in clearing bacteria or clinical signs. Therefore, early detection by the disclosed methods can improve treatment efficacy.

Also disclosed is a method for monitoring the treatment of a subject for Ehrlichiosis that comprises assaying a biological sample from the subject for levels of an antibody that specifically binds a polypeptide comprising SEQ ID NO:7, SEQ ID NO:8, or SEQ ID NO:9, or a conservative variant thereof having at least 70% identity to SEQ ID NO:7, SEQ ID NO:8, or SEQ ID NO:9. In these methods, an at least 2-, 3-, or 4-fold titer reduction in antibody levels is an indication that the treatment is effective. Of course, with chronic stage disease, this can take several months. Therefore, the method can involve assaying a sample from the subject every 1, 2, 3, 4, 5, or 6 weeks to monitor the treatment. Once antibody levels are no longer detectable, the method can further involve ceasing treatment. Alternatively, if antibody levels do not decrease as expected, then the method can further comprising altering the treatment, such as by increasing dosages or selecting an alternative antibiotic.

Also disclosed is a method for delivering a therapeutic or diagnostic agent to a cell in a subject that involves conjugating the agent, or a delivery vehicle comprising the agent, to a EtpE-C polypeptide. For example, the method can comprise administering to the subject a composition comprising the agent, wherein the agent, or a delivery vehicle comprising the agent, is conjugated to a delivery polypeptide comprising an amino acid sequence having at least 70% identity to SEQ ID NO:2, SEQ ID NO:4, SEQ ID NO:6, or a fragment thereof capable of binding DNase X, or to a nucleic acid encoding the polypeptide operably linked to a promoter. In these embodiments, the polypeptide can comprise at least 100, 101, 102, 103, 104, 105, 110, 120, 130, 140,150, 160, 170, 180, 190, or 200 amino acids of SEQ ID NO:2, SEQ ID NO:4, or SEQ ID NO:6. In some embodiments, the polypeptide comprises at least residues 1658 to 1761 of SEQ ID NO:1, or a conservative variant thereof. In some embodiments, the polypeptide comprises at least residues 1408 to 1510 of SEQ ID NO:3, or a conservative variant thereof. In some embodiments, the polypeptide comprises at least residues 1410 to 1510 of SEQ ID NO:5, or a conservative variant thereof. The disclosed method can be used to deliver the agent to any cell expressing DNase X. In addition to leukocyte, endothelial cells, and kidney cells, DNase X is highly expressed in heart, brain, and placenta. Cells from these tissues can be targeted for EtpE-C-DNase X-mediated gene or drug delivery.

The details of one or more embodiments of the invention are set forth in the accompanying drawings and the description below. Other features, objects, and advantages of the invention will be apparent from the description and drawings, and from the claims.

DESCRIPTION OF DRAWINGS

FIGS. 1A-1F show that EtpE-C is exposed at the bacterial surface, and anti-EtpE-C neutralizes E. chaffeensis infection in vitro. FIG. 1A is a Western blot analysis of E. chaffeensis-infected (Ech) and uninfected DH82 cells at 60 h pi using anti-EtpE-N (a-EtpE-N) and anti-EtpE-C (a-EtpE-C). FIG. 1B shows double immunofluorescence labeling of E. chaffeensis-infected human primary macrophages derived from peripheral blood monocytes at 56 h pi. Cells were fixed with PFA, permeabilized with saponin, and labeled with anti-EtpE-C and anti-E. chaffeensis major outer membrane protein P28. The white dashed line denotes the macrophage contour. The boxed region indicates the area enlarged in the smaller panels to the right. Merge/DIC: Fluorescence images merged with Differential interference contrast image (DIC). A single z-plane (0.4 mm thickness) by deconvolution microscopy was shown. Scale bar, 2 mm. FIG. 1C shows E. chaffeensis incubated with DH82 cells for 30 min and double immunofluorescence labeled using anti-EtpE-C and anti-E. chaffeensis P28 without permeabilization. DAPI was used to label DNA. Scale bar, 1 mm. FIG. 1D is a bar graph showing numbers of E. chaffeensis bound to RF/6A cells at 30 min pi. Host cell-free E. chaffeensis was pretreated with anti-EtpE-C or preimmune mouse serum and incubated with RF/6A cells for 30 min. Unbound E. chaffeensis was washed away, cells were fixed with PFA, and E. chaffeensis labeled with anti-P28 without permeabilization. E. chaffeensis in 100 cells were scored. FIG. 1E is a bar graph showing numbers of E. chaffeensis internalized into RF/6A cells at 2 h pi. E. chaffeensis was pretreated with anti-rEtpE-C or preimmune mouse serum and incubated with RF/6A cells for 2 h. To distinguish intracellular from bound E. chaffeensis, unbound E. chaffeensis was washed away and cells were processed for two rounds of immunostaining with anti-P28; first without permeabilization to detect bound but not internalized E. chaffeensis (AF555-conjugated secondary antibody) and second round with saponin permeabilization to detect total E. chaffeensis, i.e., bound plus internalized (AF488-conjugated secondary antibody). E. chaffeensis in 100 cells was scored. The black bar represents total E. chaffeensis and the white bar represents internalized E. chaffeensis (total minus bound) (see also FIG. 9). FIG. 1F is a bar graph showing qPCR for E. chaffeensis 16S rDNA in RF/6A cells infected with E. chaffeensis at 48 h pi. E. chaffeensis was pretreated with anti-EtpE-C or preimmune mouse serum and used to infect RF/6A cells; cells were harvested at 48 h pi. qPCR for E. chaffeensis 16S rDNA was normalized with G3PDH DNA. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05).

FIGS. 2A-2C show EtpE is expressed by E. chaffeensis in HME patients and infected dogs, and immunization with rEtpE-C protects mice against E. chaffeensis challenge. FIG. 2A shows SDS-PAGE analysis and GelCode Blue staining of rEtpE-N (lane 1) and rEtpE-C (lane 2) (5 mg/lane). rEtpE-N was partially cleaved after its expression in E. coli and thus is visualized as multiple bands. FIG. 2B shows Western blot analysis of rEtpE-N (lane 1) and rEtpE-C (lane 2) (5 μg/lane) with HME patient sera (ID: 72088, MRL1-22, MRL1-40) or control human serum (Control), or sera from dogs experimentally infected with E. chaffeensis (ID: CTUALJ, 3918815, 1425) or control dog serum. The relative band intensity for rEtpE-N/rEtpE-C (75 kDa and 34 kDa bands) assessed by densitometry was shown beneath the panels. FIG. 2C shows dot-plot analysis of E. chaffeensis load of the blood samples from rEtpE-C-immunized and placebo-immunized mice at 5 days after E. chaffeensis challenge. qPCR of E. chaffeensis 16S rDNA normalized to mouse G3PDH DNA. *Significantly different (P<0.05).

FIGS. 3A-3D show rEtpE-C-coated beads enter macrophages by a pathway similar to one that mediates E. chaffeensis entry. FIG. 3A is an image showing latex beads coated with rEtpE-C by anti-EtpE-C labeling under fluorescence microscopy. Scale bar, 1μm. FIG. 3B shows fluorescence and phase contrast merged images of rEtpE-C-coated beads incubated with mouse BMDMs. Cells were pretreated with DMSO (solvent control), MDC, genistein, or PI-PLC for 45 min followed by trypsin treatment to remove beads that were not internalized. Scale bar, 10 μm. FIGS. 3C and 3D are bar graphs showing numbers of internalized rEtpE-C-coated (C) and non-coated (D) beads/cell incubated with mouse BMDMs pretreated with MDC, genistein, or PI-PLC, relative to DMSO treatment (solvent control) set as 100. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05).

FIGS. 4A-4G show rEtpE-C-coated latex beads bind and enter non-phagocytic host cells. FIG. 4A shows rEtpE-C-coated beads (arrows), but not rEtpE-N, rECH0825, or rGroEL-coated beads, bind and enter HEK293 cells at 1 h pi. Scale bar, 10 μm. FIG. 4B is a bar graph showing quantitation of similar experiment as (A) by scoring beads in 100 cells. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 4C is a scanning electron micrograph of rEtpE-C-coated beads on the surface of RF/6A cells at 2 h pi. Note filopodia-like extensions embracing the beads (arrows). Scale bar, 1μm. FIG. 4D is a transmission electron micrograph of rEtpE-C-coated beads being engulfed (left panel) and internalized (right panel) into RF/6A cells at 8 h pi. Note filopodia-like extensions embracing the beads (arrow). Scale bars, 0.5 μm (left) and 1 μm (right). FIG. 4E contains fluorescence and DIC images of rEtpE-C-coated beads in RF/6A cells. RF/6A cells were pretreated with DMSO (solvent), MDC, verapamil, or genistein for 30 min at 37° C., then incubated with rEtpE-C-coated beads for 8 h in the presence of compounds, washed and treated with trypsin to remove beads bound on the surface. A single z-plane (0.4 μm thickness) by deconvolution microscopy is shown here. Scale bar, 10 μm. FIG. 4F is a bar graph showing numbers of internalized rEtpE-C-coated beads/cell of similar experiments as (E), relative to the number in DMSO treatment set as 100. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 4G contains fluorescence and DIC merged images of RF/6A cells incubated with rEtpE-C-coated beads immunostained at 1 h pi with anti-EEA1 after permeabilization. Arrows indicate beads surrounded with EEA1. The boxed region is enlarged to the right. A single z-plane (0.2 μm thickness) by deconvolution microscopy is shown here. Scale bar, 5 μm.

FIGS. 5A-5F show EtpE-C binds DNase X. FIG. 5A shows far-Western blotting of renatured rEtpE-C and rECH0825 on a nitrocellulose membrane incubated with THP-1 cell lysate. Native DNase X was detected with anti-DNase X (α-DNase X), and recombinant proteins were detected with anti-histidine-tag (α-His tag). FIG. 5B shows Western blotting of THP-1 cell lysate following affinity pull-down with rEtpE-C bound to Ni-silica matrix. Bound proteins were eluted with imidazole and labeled with a-DNase X or α-His tag. FIG. 5C shows Western blot analysis of E. chaffeensis-infected THP-1 cell lysate immunoprecipitated with anti-EtpE-C (α-EtpE-C) or control IgG. THP-1 cells were incubated with E. chaffeensis for 30 min, followed by lysis, and immunoprecipitated with α-EtpE-Cor control mouse IgG-bound protein A agarose. The precipitates were subjected to Western blotting with α-DNase X. ** DNase X, * mouse IgG heavy chain. FIG. 5D shows immunofluorescence labeling of rEtpE-C-coated latex beads incubated with RF/6A cells for 1 h with a-DNase X without permeabilization. Note a cluster of beads colocalizes with host cell-surface DNase X. Scale bar, 5 μm. FIG. 5E shows selected time-lapse images (0 to 6:38 min) of rEtpE-C-coated beads attached to RF/6A cells expressing DNase X-GFP at 4° C., and time 0 min was set upon raising the temperature to 37° C. The white dashed line denotes the RF/6A cell contour. A single z-plane (0.4 μm thickness) by deconvolution microscopy was shown. Scale bar, 2 μm. FIG. 5F shows line intensity profile analysis of rEtpE-C-beads and DNase X-GFP signal along the length of the line (slanted white line in the image 5E).

FIGS. 6A-6D show internalization of rEtpE-C-coated beads is dependent on DNase X. FIG. 6A shows immunofluorescence labeling of rEtpE-C-coated or noncoated beads incubated with human macrophages derived from peripheral blood monocytes. At 30 min pi, cells were labeled with a-DNase X without permeabilization. rEtpE-C-coated beads cluster and colocalize with DNase X on the cell surface, but non-coated beads do not. A single z-plane (0.4 μm thickness) by deconvolution microscopy was shown. Scale bar, 5 μm (see also FIG. 13). FIG. 6B is a selected image showing the orthogonal view of macrophage incubated with rEtpE-C-coated (left panel) or non-coated (right panel) beads in (A). The orthogonal view was obtained from the reconstituted 3-D view of serial z-stack images (combined z-section width of 7.2 μm). Scale bar, 5 μm. The fluorescence intensity profiles of DNase X and beads signals were shown. FIG. 6C shows fluorescence and phase contrast merged images of rEtpEC-coated and non-coated beads incubated with BMDMs from DNase X^(-/-) and wild-type mice. Cells and beads were incubated for 45 min followed by trypsin treatment to remove non-internalized beads. Scale bar, 10 μm. FIG. 6D shows numbers of internalized rEtpE-C-coated beads/cell of similar experiment as (C), relative to the number of non-coated beads set as 100. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05) (see also FIG. 14).

FIGS. 7A-7J show that DNase X mediates E. chaffeensis binding, entry, and infection. FIG. 7A shows double immunofluorescence labeling with a-P28 and a-DNase X, without permeabilization, of E. chaffeensis bound on DH82 cells at 45 min pi at MOI of 10:1. The white dashed line denotes the DH82 cell contour. The arrow indicates the area enlarged in the smaller panels to the right. DNase X at the host-cell surface clusters to bound E. chaffeensis (arrows). Scale bar, 5μm. FIG. 7B is a confocal image of double immunofluorescence labeled E. chaffeensis on human macrophages derived from peripheral blood monocytes at 30 min pi at MOI of 10:1, with a-P28 and a-DNase X without permeabilization. DNase X colocalizes with the sites of E. chaffeensis binding (arrow, the region enlarged in the smaller panels to the right). Scale bar, 5 μm. FIG. 7C shows numbers of E. chaffeensis bound to DH82 cells pretreated with a-DNase X or mouse IgG at 30 min pi. Immunofluorescence labeling with a-P28 was performed without permeabilization and the numbers of E. chaffeensis on 100 cells were scored. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 7D shows numbers of E. chaffeensis internalized into DH82 cells pretreated with a-DNase X or mouse IgG at 2 h pi. Cells were processed for two rounds of immunostaining with a-P28 as described in FIG. 1E. The black bar represents total E. chaffeensis, and the white bar represents internalized E. chaffeensis (total minus bound). E. chaffeensis in 100 cells were scored. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 7E shows E. chaffeensis load in DH82 cells pretreated with a-DNase X or mouse IgG at 48 h pi. qPCR for E. chaffeensis 16S rDNA normalized with canine G3PDH DNA. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 7F shows Western blot analysis of DNase X in HEK293 cells transfected with DNase X siRNA or scrambled control siRNA. Actin was used as a protein loading control. FIG. 7G shows E. chaffeensis load in HEK293 cells treated with DNase X siRNA or scrambled control siRNA at 48 h pi. qPCR for E. chaffeensis 16S rDNA normalized with human G3PDH DNA. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 7H is a bar graph showing numbers of total cell-associated and internalized E. chaffeensis in DNase X^(-/-) or wild-type BMDMs at 4 h pi. Cells were processed for two rounds of immunostaining with a-P28 as described in FIG. 1E. The total numbers of E. chaffeensis in 100 cells were scored. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. The black bar represents total E. chaffeensis, and the white bar represents internalized E. chaffeensis (total minus external). *Significantly different (P<0.05) FIGS. 71 and 7J show E. chaffeensis load in BMDMs from DNase X^(-/-) mice and wild-type mice at 56 h pi (I) or in the blood at 5 days post-infection from DNase X^(-/-) mice and wild-type mice (J). qPCR for E. chaffeensis 16S rDNA was performed and normalized with mouse G3PDH DNA. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05).

FIG. 8 is a schematic representation of E. chaffeensis binding and entry into mammalian cells. DNase X is enriched in the lipid raft domains of the cell membrane. Extracellular E. chaffeensis uses its surface protein EtpE C-terminal region to make initial contacts with cell surface DNase X that results in further lateral redistribution and local clustering of DNaseX at the sites of bacterial binding. This binding elicits signals that are relayed down-stream and culminated in host cytoskeletal remodeling, filopodial induction and engulfment of the bound bacteria into an early endosome into the host cell. This receptor-mediated endocytosis can be specifically disrupted by genistein, verapamil or MDC. Latex beads coated with rEtpE-C also bind to cell surface DNase X and follows a similar pattern of entry like that of E. chaffeensis.

FIG. 9 contains immunofluorescence image showing host cell-free E. chaffeensis that was either treated with pronase E or PBS control. Cells were processed for double immunostaining with anti-EtpE-C and anti-CtrA with or without saponin permeabilization as described to distinguish extracellular and internalized bacteria. When bacteria were treated with pronase E, the surface immunofluorescence staining of EtpE was abolished completely, but not that of the internal control CtrA. Scale bar, 1 μm.

FIGS. 10A-10B show that anti-EtpE-C neutralizes E. chaffeensis binding and entry into THP-1 cells, related to FIG. 1D-F. FIG. 10A is a bar graph showing numbers of E. chaffeensis (Ech) bound to THP-1 cells at 30 min pi. E. chaffeensis was pretreated with anti-EtpE-C or preimmune mouse serum and incubated with THP-1 cells for 30 min. Unbound E. chaffeensis was washed away, cells were fixed with PFA and E. chaffeensis was labeled with anti-P28 without permeabilization. E. chaffeensis in 100 cells was scored. FIG. 10B is a bar graph showing numbers of E. chaffeensis internalized into THP-1 cells at 2 h pi. Purified host cell-free E. chaffeensis was pretreated with anti-rEtpE-C or preimmune mouse serum and incubated with THP-1 cells for 2 h. To distinguish intracellular from bound E. chaffeensis, unbound E. chaffeensis was washed away, and cells were processed for two rounds of immunostaining with anti-P28: first without permeabilization to detect bound but not internalized E. chaffeensis (AF555-conjugated secondary antibody), and another round with saponin permeabilization to detect total E. chaffeensis, i.e., bound plus internalized (AF488-conjugated secondary antibody). The black bar represents total E. chaffeensis, and the white bar represents internalized E. chaffeensis (total minus bound). E. chaffeensis in 100 cells was scored. qPCR for E. chaffeensis 16S rDNA was normalized with human G3PDH DNA. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05).

FIGS. 11A-11B show that anti-P28 does not inhibit binding or uptake of E. chaffeensis by THP-1 cells, related to FIG. 1D-F. FIG. 11A is a bar graph showing relative radioactivity representing numbers of E. chaffeensis bound to THP-1 cells. Host cell-free radiolabeled E. chaffeensis preincubated with Fab fragment of rabbit anti-P28 IgG or pre-immune rabbit IgG were incubated with THP-1 cells for 2 h at 4° C. Unbound E. chaffeensis was washed away, and radioactivity of bound E. chaffeensis was measured. FIG. 11B is a bar graph showing relative radioactivity representing numbers of E. chaffeensis internalized into THP-1 cells. Host cell-free radiolabeled E. chaffeensis preincubated with Fab fragment of rabbit anti-P28 IgG or pre-immune rabbit IgG was incubated with THP-1 cells for 3 h at 37° C. Bound uninternalized E. chaffeensis was removed by pronase E treatment, radioactivity of internalized E. chaffeensis measured. Data represent the mean and standard deviation of triplicate samples and are representative of two independent experiments.

FIGS. 12A-12B show that anti-EtpE-N is not effective in neutralizing E. chaffeensis infection in vitro and N-terminus of EtpE is less surface-accessible in live E. chaffeensis than its C-terminus, related to FIG. 1. FIG. 12A is a bar graph showing E. chaffeensis 16S rDNA in RF/6A cells infected with E. chaffeensis. E. chaffeensis was pretreated with anti-EtpE-N or preimmune rabbit serum and used to infect RF/6A cells; cells were harvested at 48 h pi. qPCR for E. chaffeensis 16S rDNA was normalized with monkey G3PDH DNA. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05). FIG. 12B shows immunofluorescence labeling of live host cell-free E. chaffeensis. Unfixed E. chaffeensis was first incubated with anti-EtpE-C, EtpE-N, or P28 (ECHP28); then fixed and labeled with AF555-conjugated secondary antibodies. Scale bar, 10 μm.

FIG. 13 shows that MDC blocks entry of E. chaffeensis into nonphagocytic RF/6A cells, related to FIG. 4E. Immunofluorescence labeling of E. chaffeensis incubated with RF/6A cells pretreated with MDC or DMSO control. At 3 h pi, cells were treated with trypsin to remove un-internalized E. chaffeensis and then labeled with anti-P28. Scale bar, 10 μm. Bar graph shows quantitation by scoring E. chaffeensis (Ech) in 100 cells (right panel). Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05).

FIGS. 14A-14B show that rEtpE-C-coated beads recruit DNase X to the areas of binding, related to FIG. 6. rEtpE-C-coated or noncoated latex beads were incubated with canine primary macrophages derived from peripheral blood monocytes (A) or DH82 cells (B) at 37° C. for 30 min, and labeled with anti-DNase X without permeabilization. rEtpE-C-coated beads recruited surface exposed DNase X to their sites of binding and clustered, whereas non-coated beads did not colocalize with DNase X on the cell surface. A single z-plane, of an optical section thickness of 0.4-μm, at cell surface by deconvolution microscopy was shown. Scale bar, 5 μm.

FIGS. 15A-15B show that binding of rEtpE-C-coated beads is dependent on DNase X, related to FIG. 6C and D. FIG. 15A contains fluorescence and DIC merged images of rEtpE-C-coated, rECH0825-coated and non-coated beads incubated with BMDMs from wild-type and DNase X^(-/-) mice. Beads were incubated with cells for 30 min at 4° C. followed by rigorous washing with PBS to remove unbound or loosely-adherent beads. Scale bar, 5 μm. FIG. 15B is a bar graph showing numbers of internalized rEtpE-C-coated beads/cell of similar experiment as (A), relative to the number of rECH0825-coated beads bound to wild-type BMDM set as 100. Data represent the mean and standard deviation of triplicate samples and are representative of three independent experiments. *Significantly different (P<0.05).

DETAILED DESCRIPTION

The comparative genome hybridization study of E. chaffeensis strains revealed that a hypothetical protein, ECH1038, consists of highly conserved N- and C-terminal segments flanking its strain-variable central region. ECH1038 expression is up-regulated in the DC stage of E. chaffeensis. As disclosed herein, ECH1038 (here named as entry triggering protein of Ehrlichia, EtpE), particularly its C-terminal conserved region (EtpE-C), is critical for E. chaffeensis binding, entry, and infection of several different host cell types. DNase X, a host cell surface GPI-anchored protein, is the receptor of EtpE-C mediating the entry of E. chaffeensis into several mammalian cell types permissive to its replication. Moreover, immunization with rEtpE-C is also shown herein to protect mice against Ehrlichia sp. challenge. Further, antibodies to both the EtpE-C and the N-terminal region (“EtpE-N”) can be found in subjects infected with Ehrlichia sp. Importantly, the EtpE-N is highly conserved across Ehrlichia sp. Therefore, disclosed herein are vaccines, diagnostics, and cell delivery polypeptides and uses therefore that take advantage of these unique properties of EtpEs.

Immunogenic polypeptides are disclosed that contain all or part of an EtpE protein from an Ehrlichia sp. This encompasses active fragments and variants of the immunogenic polypeptide. Thus, the term “immunogenic or antigenic polypeptide” further contemplates deletions, additions and substitutions to the disclosed sequences, so long as the polypeptide functions to produce an immunological response as defined herein.

For example, the immunogenic polypeptide can comprise the amino acid sequence SEQ ID NO:1 (EtpE from Ehrlichia chaffeensis str. Arkansas; Accession No. YP_507823.1), SEQ ID NO:3 (EtpE from Ehrlichia canis str. Jake; Accession No. AAZ68869.1), or SEQ ID NO:5 (EtpE from Ehrlichia ruminantium str. Welgevonden; Accession No. YP_180660.1). EtpE homologues from other Ehrlichia sp. can also be identified and used to improve species cross-reactivity.

Importantly, genome sequencing has resulted in nomenclature changes and in some cases reclassification of both genus and species in the past. It is therefore possible, that members of the Ehrlichia genus could be reclassified as a different species sometime in the future. Less likely, but still possible, is the future reclassification of a species in or out of the Ehrlichia genus. Therefore, while reference to species and genus is meaningful, it is also understood that genus classification is less important than the presence of homologoues/orthologous EtpE proteins in the related organism, which can be identified and confirmed independently from genus/species classification.

In some embodiments, the vaccine contains an immunogenic fragment of an EtpE protein that is capable of eliciting an immune response against an Ehrlichia sp. Preferably, the immunogenic fragment comprises at least a portion of the conserved region (“EtpE-C”). For example, the one or more polypeptide can comprise the amino acid sequence SEQ ID NO:2 (residues 1656-1963 of SEQ ID NO:1), SEQ ID NO:4 (residues 1408-1510 of SEQ ID NO:3), SEQ ID NO:6 (residues 1410-1710 of SEQ ID NO:5), or a an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp.

The vaccine can alternatively contain an immunogenic variant of an EtpE protein, or fragment thereof, that is capable of eliciting an immune response against an Ehrlichia sp. For example, the vaccine can comprise one or more polypeptides having an amino acid sequence with at least 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100% identity to an amino acid sequence selected from the group consisting of SEQ ID NO:1, SEQ ID NO:3, SEQ ID NO:5, or an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp. The vaccine can comprise one or more polypeptides having an amino acid sequence with at least 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100% identity to SEQ ID NO:2, SEQ ID NO:4, SEQ ID NO:6, or a an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp.

The vaccine comprises polypeptides representing the EtpE from at least one Ehrlichia sp. However, to improve cross-reactivity, the vaccine can contain polypeptides representing the EtpE from at least 2, 3, 4, 5, 6, or more Ehrlichia sp. These polypeptides can be in a single amino acid sequence, such as fusion protein. The polypeptides can also be conjugated together on a single carrier molecule. For example, the polypeptides can be used in a multiple antigen peptide system (MAPS).

Fusion proteins, also known as chimeric proteins, are proteins created through the joining of two or more genes which originally coded for separate proteins. Translation of this fusion gene results in a single polypeptide with function properties derived from each of the original proteins. Recombinant fusion proteins can be created artificially by recombinant DNA technology for use in biological research or therapeutics. Chimeric mutant proteins occur naturally when a large-scale mutation, typically a chromosomal translocation, creates a novel coding sequence containing parts of the coding sequences from two different genes.

A recombinant fusion protein is a protein created through genetic engineering of a fusion gene. This typically involves removing the stop codon from a cDNA sequence coding for the first protein, then appending the cDNA sequence of the second protein in frame through ligation or overlap extension PCR. That DNA sequence will then be expressed by a cell as a single protein. The protein can be engineered to include the full sequence of both original proteins, or only a portion of either.

If the two entities are proteins, often linker (or “spacer”) peptides are also added which make it more likely that the proteins fold independently and behave as expected. Especially in the case where the linkers enable protein purification, linkers in protein or peptide fusions are sometimes engineered with cleavage sites for proteases or chemical agents which enable the liberation of the two separate proteins. This technique is often used for identification and purification of proteins, by fusing a GST protein, FLAG peptide, or a hexa-his peptide (aka: a6xhis-tag) which can be isolated using nickel or cobalt resins (affinity chromatography). Chimeric proteins can also be manufactured with toxins or anti-bodies attached to them in order to study disease development.

Alternatively, internal ribosome entry sites (IRES) elements can be used to create multigene, or polycistronic, messages. IRES elements are able to bypass the ribosome scanning model of 5′ methylated Cap dependent translation and begin translation at internal sites. IRES elements can be linked to heterologous open reading frames. Multiple open reading frames can be transcribed together, each separated by an IRES, creating polycistronic messages. By virtue of the IRES element, each open reading frame is accessible to ribosomes for efficient translation. Multiple genes can be efficiently expressed using a single promoter/enhancer to transcribe a single message.

In some embodiments, the vaccine is capable of eliciting an immune response against at least Ehrlichia chaffeensis. In these embodiments at least one of the one or more polypeptides comprise SEQ ID NO:1, SEQ ID NO:2, or an immunogenic variant or fragment thereof capable of eliciting an immune response against Ehrlichia chaffeensis.

In some embodiments, the vaccine is capable of eliciting an immune response against at least Ehrlichia canis. In these embodiments at least one of the one or more polypeptides comprise SEQ ID NO:3 or an immunogenic variant or fragment thereof capable of eliciting an immune response against Ehrlichia canis.

In some embodiments, the vaccine is capable of eliciting an immune response against at least Ehrlichia ruminantium. In these embodiments at least one of the one or more polypeptides comprise SEQ ID NO:5 or an immunogenic variant or fragment thereof capable of eliciting an immune response against Ehrlichia ruminantium.

In some embodiments, the vaccine is capable of eliciting an immune response against any combination of Ehrlichia chaffeensis, Ehrlichia canis, and Ehrlichia ruminantium. The vaccine can also be capable of eliciting an immune response against other species, such as Ehrlichia muris, Ehrlichia ewingii, or a combination thereof. The EtpE homologue from these and other species and strains can be identified and used as immunogens as described herein.

Adjuvants suitable for use with the disclosed vaccine are known and include Quil A, aluminum salts, squalene, virosomes, and combinations thereof. Likewise, immune stimulants suitable for use with the disclosed vaccine are known and include cytokines, growth factors, chemokines, and combinations thereof.

Also disclosed is a recombinant vector that contains a nucleic acid sequence encoding any of the one or more immunogenic polypeptides disclosed herein, operatively linked to a heterologous promoter. Suitable vectors for propagating and/or expressing the nucleic acid sequence encoding any of the one or more immunogenic polypeptides are known in the art. In some embodiments, the vector is a plasmid selected from the group consisting of pcDNA3, pCI, VR1020, VR1012, and VR1055. These are mammalian expression plasmids which usually consist of a strong viral promoter to drive the in vivo transcription and translation of the gene (or complementary DNA) and include a strong polyadenylation/transcriptional termination signal. For example, VR1055 vector contains HCMV promotor, intron A (to improve mRNA stability) and multicloning site, mRBG (minimal rabbit globin terminator) and kanamycin selection marker. A bacterial DNA sequence codon-optimized for mammalian expression is inserted at the multicloning site.

In some embodiments, the vector is a recombinant viral vector. For example, the recombinant viral vector can be selected from the group consisting of poxvirus, adenovirus, adeno-associated virus, lentivirus, and herpesvirus. A live virus vector vaccine uses a weakened replication defective virus to transport genes encoding bacterial DNA sequence to elicit immune response to the bacterial protein. For example, a modified ACAM2000 vaccinia virus (VACV) that is further reduced of its virulence potential through deletion of thymidine kinase (TK; J2R) and IL-18 binding protein (IL18BP; C12L). The inactivation of the TK gene greatly reduces VACV virulence. In fact, a TK-null VACV, JX-594, was shown to be safe as an oncolytic virus for cancer patients in phase I clinical trial. Since viral envelop proteins elicit strong B- and T-cell immune responses, a fusion protein of viral envelop protein such as D8 and the bacterial protein is constructed and inserted into viral genome to produce a recombinant virus.

Suitable promoters for driving expression of nucleic acids encoding the disclosed polypeptides are also known and can be selected, for example, from the group consisting of human or murine cytomegalovirus major immediate early (IE) promoter (CMV-IE), the early/late promoter of the SV40 virus, and the LTR promoter of the Rous sarcoma virus. In some embodiments, a viral promoter can be used to drive a downstream gene encoding a fusion between a part of viral protein (for example, the transmembrane domain of D8 of VACV and EtpE-C (codon optimized).

Also disclosed is a vaccine containing any of the disclosed recombinant vectors in a pharmaceutically acceptable vehicle, diluent or excipient. The vaccine can further contain a pharmaceutically acceptable adjuvant. Suitable adjuvants for use with DNA vaccines are known and include, for example, an oligonucleotide comprising a CpG motif, or a vector encoding one or more growth factors, cytokines, chemokine, or combination thereof. For example, the growth factor can be granulocyte macrophage colony-stimulating factor (GM-CSF).

Also disclosed is a method for vaccinating a subject against Ehrlichia sp, that comprises administering to the subject a composition comprising any of the disclosed vaccines. The subject can be any mammal at risk for Ehrlichia sp. infection. In particular, the subject can be a human, canine, feline, bovine, ovine, or caprine subject. The method provides a protective immune response against at least one Ehrlichia sp. selected from the group consisting of Ehrlichia chaffeensis, Ehrlichia canis, and Ehrlichia ruminantium. However, in preferred embodiments, the vaccine elicits a protective immune response in the subject against at least 2, 3, 4, 5, 6, or more Ehrlichia sp.

Also disclosed is a method for diagnosing Ehrlichiosis in a subject that comprising assaying a biological sample (e.g., blood, serum, or plasma sample) from the subject for the presence of an antibody that specifically binds an EtpE polypeptide. In particular, assaying for antibodies that specifically bind an EtpE-N provides pan-diagnosis of Ehrlichia sp. infection since the N-terminal domain is highly conserved across species. Therefore, in some embodiments, the presence of the antibody is an indication that the subject has been infected with an Ehrlichia sp. selected from the group consisting of Ehrlichia chaffeensis, Ehrlichia canis, Ehrlichia ruminantium, or any combination thereof. Therefore, the method can involve assaying a biological sample from the subject for the presence of an antibody that specifically binds SEQ ID NO:7 (amino acid residues 29-708 of SEQ ID NO:1), SEQ ID NO:8 (amino acid residues 73-736 of SEQ ID NO:3), SEQ ID NO:9 (amino acid residues 39-730 of SEQ ID NO:5), or a conservative variant thereof having at least 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100% identity to SEQ ID NO:7, SEQ ID NO:8, or SEQ ID NO:9, wherein the presence of the antibody is an indication that the subject has been infected with an Ehrlichia sp.

In some aspects, the method is an immunoassay. Many types and formats of immunoassays are known and all are suitable for detecting the disclosed biomarkers. Examples of immunoassays are enzyme linked immunosorbent assays (ELISAs), radioimmunoassays (RIA), radioimmune precipitation assays (RIPA), immunobead capture assays, Western blotting, dot blotting, gel-shift assays, Flow cytometry, protein arrays, multiplexed bead arrays, magnetic capture, in vivo imaging, fluorescence resonance energy transfer (FRET), and fluorescence recovery/localization after photobleaching (FRAP/ FLAP).

In some embodiments, the method provides a pan-diagnostic so that one test can be used for multiple species of Ehrlichia. However, in some embodiments, the method also diagnoses the specific Ehrlichia sp. In these embodiments, the EtpE-C polypeptide can be used to detect antibodies that selectively bind the C-terminal region of an EtpE from a specific species of Ehrlichia. This is useful since prognosis (choronic vs. acute disease) and zoonotic potential are different depending on the species of Ehrlichia. Although all of these species can infect humans, levels of zoonosis potential is in the order of E. chaffeensis>E. ewinigil>E. muris>E. canis>E. ruminantium. E. chaffeensis infection in humans is acute, and can be fatal. E. canis infection is chronic and debilitating febrile illness in dogs (infection for life if not treated at early stage of infection). Clinical signs of E. canis infection in humans is generally mild, but can be severe. E. canis can also infect cats, and clinical signs of cats are similar to those in infected dogs. E. ewingii infection in humans is acute, and some case is associated with infection of pet dogs (E. chaffeensis is not, since its major reservoir is wild deer). E. ewingii infection of dogs is chronic. Wild rodents are the reservoir of E. muris (chronic infection), and clinical signs of human infection without underlining other diseases is relatively mild, and has been transmitted between humans via blood transfusion of contaminated blood. E. ruminantium causes acute and chronic debilitating disease accompanied with neurological signs (heart water, often fatal) of ruminants (cattle, goat, sheep) in Africa and Caribbean countries. Only rare cases of human infection with E. ruminantium (severe, acute) have been reported.

The disclosed methods can further comprise treating the subject for Ehrlichiosis if the antibody is detected. For example, the method can comprise treating the subject with an effective amount and duration of doxycycline if the antibody is detected. This should be done as early as possible, since at later stage of infection antibiotic becomes less effective in clearing bacteria or clinical signs. Therefore, early detection by the disclosed methods can improve treatment efficacy.

Also disclosed is a method for monitoring the treatment of a subject for Ehrlichiosis that comprises assaying a biological sample from the subject for levels of an antibody that specifically binds a polypeptide comprising SEQ ID NO:7, SEQ ID NO:8, or SEQ ID NO:9, or a conservative variant thereof having at least 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100% identity to SEQ ID NO:7, SEQ ID NO:8, or SEQ ID NO:9. In these methods, an at least 2-, 3-, or 4-fold titer reduction in antibody levels is an indication that the treatment is effective. Of course, with chronic stage disease, this can take several months. Therefore, the method can involve assaying a sample from the subject every 1, 2, 3, 4, 5, or 6 weeks to monitor the treatment. Once antibody levels are no longer detectable, the method can further involve ceasing treatment. Alternatively, if antibody levels do not decrease as expected, then the method can further comprising altering the treatment, such as by increasing dosages or selecting an alternative antibiotic.

Also disclosed is a method for delivering a therapeutic or diagnostic agent to a cell in a subject that involves conjugating the agent, or a delivery vehicle comprising the agent, to a EtpE-C polypeptide. For example, the method can comprise administering to the subject a composition comprising the agent, wherein the agent, or a delivery vehicle comprising the agent, is conjugated to a delivery polypeptide comprising an amino acid sequence having at least 70%, 71%, 72%, 73%, 74%, 75%, 76%, 77%, 78%, 79%, 80%, 81%, 82%, 83%, 84%, 85%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99%, or 100% identity to SEQ ID

NO:2, SEQ ID NO:4, SEQ ID NO:6, or a fragment thereof capable of binding DNase X, or to a nucleic acid encoding the polypeptide operably linked to a promoter.

In some embodiments, the polypeptide comprises at least 100, 101, 102, 103, 104, 105, 110, 120, 130, 140,150, 160, 170, 180, 190, or 200 amino acids of SEQ ID NO:2, SEQ ID NO:4, or SEQ ID NO:6.

In some embodiments, the polypeptide comprises at least residues 1658 to 1761 of SEQ ID NO:1, including residues 1658 to 1761, 1762, 1763, 1764, 1765, 1766, 1767, 1768, 1769, 1770, 1771, 1772, 1773, 1774, 1775, 1776, 1777, 1778, 1779, 1780, 1781, 1782, 1783, 1784, 1785, 1786, 1787, 1788, 1789, 1790, 1791, 1792, 1793, 1794, 1795, 1796, 1797, 1798, 1799, 1800, 1801, 1802, 1803, 1804, 1805, 1806, 1807, 1808, 1809, 1810, 1811, 1812, 1813, 1814, 1815, 1816, 1817, 1818, 1819, 1820, 1821, 1822, 1823, 1824, 1825, 1826, 1827, 1828, 1829, 1830, 1831, 1832, 1833, 1834, 1835, 1836, 1837, 1838, 1839, 1840, 1841, 1842, 1842, 1844, 1845, 1846, 1847, 1848, 1849, 1850, 1851, 1852, 1853, 1854, 1855, 1856, 1857, 1858, 1859, 1860, 1861, 1862, 1863, 1864, 1865, 1866, 1867, 1868, 1869, 1870, 1871, 1872, 1873, 1874, 1875, 1876, 1877, 1878, 1879, 1880, 1881, 1882, 1883, 1884, 1885, 1886, 1887, 1888, 1889, 1890, 1891, 1892, 1893, 1894, 1895, 1896, 1897, 1898, 1899, 1900, 1901, 1902, 1903, 1904, 1905, 1906, 1907, 1908, 1910, 1911, 1912, 1913, 1914, 1915, 1916, 1917, 1918, 1919, 1920, 1921, 1922, 1923, 1924, 1925, 1926, 1927, 1928, 1929, 1930, 1931, 1932, 1933, 1934, 1935, 1936, 1937, 1938, 1939, 1940, 1941, 1942, 1943, 1944, 1945, 1946, 1947, 1948, 1949, 1950, 1951, 1952, 1953, 1954, 1955, 1956, 1957, 1958, 1959, 1960, 1961, 1962, or 1963 of SEQ ID NO:1, or a conservative variant thereof.

In some embodiments, the polypeptide comprises at least residues 1408 to 1510 of SEQ ID NO:3. In some embodiments, the polypeptide comprises at least residues 1410 to 1510 of SEQ ID NO:5, including residues 1408 to 1510,

1511, 1512, 1513, 1514, 1515, 1516, 1517, 1518, 1519, 1520, 1521, 1522, 1523, 1524, 1525, 1526, 1527, 1528, 1529, 1530, 1531, 1532, 1533, 1534, 1535, 1536, 1537, 1538, 1539, 1540, 1541, 1542, 1542, 1544, 1545, 1546, 1547, 1548, 1549, 1550, 1551, 1552, 1553, 1554, 1555, 1556, 1557, 1558, 1559, 1560, 1561, 1562, 1563, 1564, 1565, 1566, 1567, 1568, 1569, 1570, 1571, 1572, 1573, 1574, 1575, 1576, 1577, 1578, 1579, 1580, 1581, 1582, 1583, 1584, 1585, 1586, 1587, 1588, 1589, 1590, 1591, 1592, 1593, 1594, 1595, 1596, 1597, 1598, 1599, 1600, 1601, 1602, 1603, 1604, 1605, 1606, 1607, 1608, 1610, 1611, 1612, 1613, 1614, 1615, 1616, 1617, 1618, 1619, 1620, 1621, 1622, 1623, 1624, 1625, 1626, 1627, 1628, 1629, 1630, 1631, 1632, 1633, 1634, 1635, 1636, 1637, 1638, 1639, 1640, 1961, 1662, 1663, 1644, 1645, 1646, 1647, 1648, 1649, 1650, 1651, 1652, 1653, 1654, 1655, 1656, 1657, 1658, 1659, 1660, 1661, 1662, 1663, 1664, 1665, 1666, 1667, 1668, 1669, 1670, 1671, 1672, 1673, 1674, 1675, 1676, 1677, 1678, 1679, 1680, 1681, 1682, 1683, 1684, 1685, 1686, 1687, 1688, 1689, 1690, 1691, 1692, 1693, 1694, 1695, 1696, 1697, 1698, 1699, 1700, 1701, 1702, 1703, 1704, 1705, 1706, 1707, 1708, 1709, or 1710 of SEQ ID NO:5.

The therapeutic or diagnostic agent can be any pharmaceutically acceptable substance for which delivery to a cell in a subject is desired. The agent can be a therapeutic drug (e.g., small molecule) or biologic (e.g., antibody, peptide, growth factor). The diagnostic agent can be a molecule detectable in the body of a subject by an imaging technique such as X-ray radiography, ultrasound, computed tomography (CT), single-photon emission computed tomography (SPECT), magnetic resonance imaging (MRI), positron emission tomography (PET), Optical Fluorescent Imaging, Optical Visible light imaging, and nuclear medicine including Cerenkov Light Imaging. For example, the diagnostic agent can comprise a radionuclide, paramagnetic metal ion, or a fluorophore. Fluorophores emit energy throughout the visible spectrum; however, the best spectrum for in vivo imaging is in the near-infrared (NIR) region (650 nm-900 nm). Unlike the visible light spectrum (400-650 nm), in the NIR region, light scattering decreases and photo absorption by hemoglobin and water diminishes, leading to deeper tissue penetration of light. Furthermore, tissue auto-fluorescence is low in the NIR spectra, which allows for a high signal to noise ratio. There is a range of small molecule organic fluorophores with excitation and emission spectra in the NIR region. Some, such as indocyanine green (ICG) and cyanine derivatives Cy5.5 and Cy7, have been used in imaging for a relatively long time. Modern fluorophores are developed by various biotechnology companies and include: Alexa dyes; IRDye dyes; VivoTag dyes and HylitePlus dyes. In general, the molecular weights of these fluorophores are below 1 kDa. In some embodiments, the diagnostic agent comprises a radiocontrast agent. Examples of suitable radiocontrast agents include iohexol, iodixanol and ioversol.

The disclosed delivery polypeptide can be conjugated to agents using known techniques, depending on the type of agent selected. For example, where the agent is a polypeptide, the composition can be a fusion protein that contains both the agent and the delivery polypeptide. Likewise, the composition can comprises a DNA expression vector encoding a fusion protein comprising the agent and the delivery polypeptide operably linked to a promoter. In some embodiments, the composition comprises a nanoparticle, microparticle, or microsphere encapsulating the agent. In these embodiments, the delivery polypeptide can be positioned on the surface of the nanoparticle, microparticle, or microspheres to facilitate delivery. For example, the microsphere can comprise lactide-co-glycoid or a polyanhydride. In some embodiments, the composition comprises a biodegradable polymer conjugated to the delivery polypeptide.

The disclosed method can be used to deliver the agent to any cell expressing DNase X. In addition to leukocyte, endothelial cells, and kidney cells, DNase X is highly expressed in heart, brain, and placenta. Cells from these tissues can be targeted for EtpE-C-DNase X-mediated gene or drug delivery. A key premise for the success of cardiac gene therapy is the development of powerful gene transfer vehicles that can achieve highly efficient and persistent gene transfer specifically in the heart. For example, the delivery mechanism can be used to deliver vascular endothelial growth factor DNA to stimulate stem cells of cardiac and skeletal muscles in vivo or to grow the cells in cell culture system to transplant matured muscle cells to regenerate the damaged tissue. Leukemia cells can be treated through autologous transplantation of hematopoietic stem cells gene-modified in vitro by delivering a normal gene into hematopoietic stem cells.

Disclosed are pharmaceutical compositions containing therapeutically effective amounts of one or more of the disclosed polypeptides, nucleic acids, or vaccines and a pharmaceutically acceptable carrier. The phrase “pharmaceutically acceptable” is employed herein to refer to those compounds, materials, compositions, and/or dosage forms which are, within the scope of sound medical judgment, suitable for use in contact with the tissues of human beings and animals without excessive toxicity, irritation, allergic response, or other problems or complications commensurate with a reasonable benefit/risk ratio. Pharmaceutical carriers suitable for administration of the molecules provided herein include any such carriers known to those skilled in the art to be suitable for the particular mode of administration.

The polypeptides, nucleic acids, or vaccines can be formulated for a variety of routes of administration and/or applications. Suitable dosage forms for parenteral administration include solutions, suspensions, and emulsions. Typically, the polypeptides, nucleic acids, or vaccines are dissolved or suspended in a suitable solvent such as, for example, water, Ringer's solution, phosphate buffered saline (PBS), or isotonic sodium chloride. The formulation may also be a sterile solution, suspension, or emulsion in a nontoxic, parenterally acceptable diluent or solvent such as 1,3-butanediol. Formulations may further include one or more additional excipients. Representative excipients include solvents, diluents, pH modifying agents, preservatives, antioxidants, antinfective agents, suspending agents, wetting agents, viscosity modifiers, tonicity agents, stabilizing agents, and combinations thereof. Suitable pharmaceutically acceptable excipients are preferably selected from materials which are generally recognized as safe (GRAS), and may be administered to an individual without causing undesirable biological side effects or unwanted interactions. In some cases, formulations can include one or more tonicity agents to adjust the isotonic range of the formulation. Suitable tonicity agents are well known in the art and include glycerin, mannitol, sorbitol, sodium chloride, and other electrolytes. In some cases, the formulations can be buffered with an effective amount of buffer necessary to maintain a pH suitable for parenteral administration. Suitable buffers are well known by those skilled in the art and some examples of useful buffers are acetate, borate, carbonate, citrate, and phosphate buffers. In some instances, the formulation is distributed or packaged in a liquid form. Alternatively, formulations for ocular administration can be packed as a solid, obtained, for example by lyophilization of a suitable liquid formulation. The solid can be reconstituted with an appropriate carrier or diluent prior to administration.

The exact amount of the disclosed compositions administered to a subject will vary from subject to subject, depending on the nature of the diagnostic or therapeutic agent, the species, age, weight and general condition of the subject, the mode of administration and the like. Effective dosages and schedules for administering the compositions may be determined empirically, and making such determinations is within the skill in the art. The dosage ranges for the administration of the compositions are those large enough to produce the desired effect (e.g., a therapeutic result or a suitable diagnostic result). The dosage should not be so large as to cause adverse side effects, such as unwanted cross-reactions, anaphylactic reactions, and the like. The dosage can be adjusted by the individual physician in the event of any counter indications.

The term “subject” refers to any individual who is the target of administration or treatment. The subject can be a vertebrate, for example, a mammal. Thus, the subject can be a human or veterinary patient. The term “patient” refers to a subject under the treatment of a clinician, e.g., physician.

The term “therapeutically effective” refers to the amount of the composition used is of sufficient quantity to ameliorate one or more causes or symptoms of a disease or disorder. Such amelioration only requires a reduction or alteration, not necessarily elimination.

The term “pharmaceutically acceptable” refers to those compounds, materials, compositions, and/or dosage forms which are, within the scope of sound medical judgment, suitable for use in contact with the tissues of human beings and animals without excessive toxicity, irritation, allergic response, or other problems or complications commensurate with a reasonable benefit/risk ratio.

The term “sample from a subject” refers to a tissue (e.g., tissue biopsy), organ, cell (including a cell maintained in culture), cell lysate (or lysate fraction), biomolecule derived from a cell or cellular material (e.g. a polypeptide or nucleic acid), or body fluid from a subject. Non-limiting examples of body fluids include blood, urine, plasma, serum, tears, lymph, bile, cerebrospinal fluid, interstitial fluid, aqueous or vitreous humor, colostrum, sputum, amniotic fluid, saliva, anal and vaginal secretions, perspiration, semen, transudate, exudate, and synovial fluid.

The term “treatment” refers to the medical management of a patient with the intent to cure, ameliorate, stabilize, or prevent a disease, pathological condition, or disorder. This term includes active treatment, that is, treatment directed specifically toward the improvement of a disease, pathological condition, or disorder, and also includes causal treatment, that is, treatment directed toward removal of the cause of the associated disease, pathological condition, or disorder. In addition, this term includes palliative treatment, that is, treatment designed for the relief of symptoms rather than the curing of the disease, pathological condition, or disorder; preventative treatment, that is, treatment directed to minimizing or partially or completely inhibiting the development of the associated disease, pathological condition, or disorder; and supportive treatment, that is, treatment employed to supplement another specific therapy directed toward the improvement of the associated disease, pathological condition, or disorder.

The terms “peptide,” “protein,” and “polypeptide” are used interchangeably to refer to a natural or synthetic molecule comprising two or more amino acids linked by the carboxyl group of one amino acid to the alpha amino group of another.

The term “protein domain” refers to a portion of a protein, portions of a protein, or an entire protein showing structural integrity; this determination may be based on amino acid composition of a portion of a protein, portions of a protein, or the entire protein.

The term “nucleic acid” refers to a natural or synthetic molecule comprising a single nucleotide or two or more nucleotides linked by a phosphate group at the 3′ position of one nucleotide to the 5′ end of another nucleotide. The nucleic acid is not limited by length, and thus the nucleic acid can include deoxyribonucleic acid (DNA) or ribonucleic acid (RNA).

A “fusion protein” refers to a polypeptide formed by the joining of two or more polypeptides through a peptide bond formed between the amino terminus of one polypeptide and the carboxyl terminus of another polypeptide. The fusion protein can be formed by the chemical coupling of the constituent polypeptides or it can be expressed as a single polypeptide from nucleic acid sequence encoding the single contiguous fusion protein. A single chain fusion protein is a fusion protein having a single contiguous polypeptide backbone. Fusion proteins can be prepared using conventional techniques in molecular biology to join the two genes in frame into a single nucleic acid, and then expressing the nucleic acid in an appropriate host cell under conditions in which the fusion protein is produced.

The term “specifically deliver” as used herein refers to the preferential association of a molecule with a cell or tissue bearing a particular target molecule or marker and not to cells or tissues lacking that target molecule. It is, of course, recognized that a certain degree of non-specific interaction may occur between a molecule and a non- target cell or tissue. Nevertheless, specific delivery, may be distinguished as mediated through specific recognition of the target molecule. Typically specific delivery results in a much stronger association between the delivered molecule and cells bearing the target molecule than between the delivered molecule and cells lacking the target molecule.

The term “vector” refers to a replicon, such as a plasmid, phage, or cosmid, into which another DNA segment may be inserted so as to bring about the replication of the inserted segment. The vectors can be expression vectors.

The term “expression vector” refers to a vector that includes one or more expression control sequences

The term “operably linked to” refers to the functional relationship of a nucleic acid with another nucleic acid sequence. Promoters, enhancers, transcriptional and translational stop sites, and other signal sequences are examples of nucleic acid sequences operably linked to other sequences. For example, operable linkage of DNA to a transcriptional control element refers to the physical and functional relationship between the DNA and promoter such that the transcription of such DNA is initiated from the promoter by an RNA polymerase that specifically recognizes, binds to and transcribes the DNA.

The terms “transformation” and “transfection” mean the introduction of a nucleic acid, e.g., an expression vector, into a recipient cell including introduction of a nucleic acid to the chromosomal DNA of said cell.

As used herein, the term “amino acid sequence” refers to a list of abbreviations, letters, characters or words representing amino acid residues. The amino acid abbreviations used herein are conventional one letter codes for the amino acids and are expressed as follows: A, alanine; B, asparagine or aspartic acid; C, cysteine; D aspartic acid; E, glutamate, glutamic acid; F, phenylalanine; G, glycine; H histidine; I isoleucine; K, lysine; L, leucine; M, methionine; N, asparagine; P, proline; Q, glutamine; R, arginine; S, serine; T, threonine; V, valine; W, tryptophan; Y, tyrosine; Z, glutamine or glutamic acid. As used herein, “peptidomimetic” means a mimetic of a peptide which includes some alteration of the normal peptide chemistry. Peptidomimetics typically enhance some property of the original peptide, such as increase stability, increased efficacy, enhanced delivery, increased half life, etc. Methods of making peptidomimetics based upon a known polypeptide sequence is described, for example, in U.S. Pat. Nos. 5,631,280; 5,612,895; and 5,579,250. Use of peptidomimetics can involve the incorporation of a non-amino acid residue with non-amide linkages at a given position. One embodiment of the present invention is a peptidomimetic wherein the compound has a bond, a peptide backbone or an amino acid component replaced with a suitable mimic. Some non-limiting examples of unnatural amino acids which may be suitable amino acid mimics include β-alanine, L-α-amino butyric acid, L-γ-amino butyric acid, L-α-amino isobutyric acid, L-ε-amino caproic acid, 7-amino heptanoic acid, L-aspartic acid, L-glutamic acid, N-ε-Boc-N-α-CBZ-L-lysine, N-ε-Boc-N-α-Fmoc-L-lysine, L-methionine sulfone, L-norleucine, L-norvaline, N-α-Boc-N-δCBZ-L-ornithine, N-δ-Boc-N-α-CBZ-L-ornithine, Boc-p-nitro-L-phenylalanine, Boc-hydroxyproline, and Boc-L-thioproline.

The term “variant” refers to an amino acid or peptide sequence having conservative amino acid substitutions, non-conservative amino acid substitutions (i.e. a degenerate variant), substitutions within the wobble position of each codon (i.e. DNA and RNA) encoding an amino acid, amino acids added to the C-terminus of a peptide, or a peptide having 60%, 70%, 80%, 90%, or 95% homology to a reference sequence.

Variants also include allelic variants. The term “allelic variant” refers to a polynucleotide or a polypeptide containing polymorphisms that lead to changes in the amino acid sequences of a protein and that exist within a natural population (e.g., a virus species or variety). Allelic variants can be identified by sequencing the nucleic acid sequence of interest in a number of different species, which can be readily carried out by using hybridization probes to identify the same gene genetic locus in those species. Any and all such nucleic acid variations and resulting amino acid polymorphisms or variations that are the result of natural allelic variation and that do not alter the functional activity of gene of interest, are intended to be within the scope of the disclosed polypeptides and nucleic acids.

The term “percent (%) sequence identity” or “homology” is defined as the percentage of nucleotides or amino acids in a candidate sequence that are identical with the nucleotides or amino acids in a reference nucleic acid sequence, after aligning the sequences and introducing gaps, if necessary, to achieve the maximum percent sequence identity. Alignment for purposes of determining percent sequence identity can be achieved in various ways that are within the skill in the art, for instance, using publicly available computer software such as BLAST, BLAST-2, ALIGN, ALIGN-2 or Megalign (DNASTAR) software. Appropriate parameters for measuring alignment, including any algorithms needed to achieve maximal alignment over the full-length of the sequences being compared can be determined by known methods.

The term “antibody” refers to natural or synthetic antibodies that selectively bind a target antigen. The term includes polyclonal and monoclonal antibodies. In addition to intact immunoglobulin molecules, also included in the term “antibodies” are fragments or polymers of those immunoglobulin molecules, and human or humanized versions of immunoglobulin molecules that selectively bind the target antigen.

The term “specifically binds”, as used herein, when referring to a polypeptide (including antibodies) or receptor, refers to a binding reaction which is determinative of the presence of the protein or polypeptide or receptor in a heterogeneous population of proteins and other biologics. Thus, under designated conditions (e.g. immunoassay conditions in the case of an antibody), a specified ligand or antibody “specifically binds” to its particular “target” (e.g. an antibody specifically binds to an endothelial antigen) when it does not bind in a significant amount to other proteins present in the sample or to other proteins to which the ligand or antibody may come in contact in an organism. Generally, a first molecule that “specifically binds” a second molecule has an affinity constant (Ka) greater than about 10⁵M⁻¹ (e.g., 10⁶M⁻¹, 10⁷M⁻¹, 10⁸M⁻¹, 10⁹M⁻¹, 10¹⁰M⁻¹, 10¹¹M⁻¹, and 10¹²M⁻¹ or more) with that second molecule.

The term “immunogenic” as used herein refers to a composition that is able to provoke an immune response against it.

The term “immune response” as used herein refers to the reaction of the immune system to the presence of an antigen by making antibodies to the antigen. In further specific embodiments, immunity to the antigen may be developed on a cellular level, by the body as a whole, hypersensitivity to the antigen may be developed, and/or tolerance may be developed, such as from subsequent challenge. In specific embodiments, an immune response entails lymphocytes identifying an antigenic molecule as foreign and inducing the formation of antibodies and lymphocytes capable of reacting with it and rendering it less harmful.

The term “immunoreactive” as used herein refers to a composition being reactive with antibodies from the sera of an individual. In specific embodiments, a composition is immunoreactive if an antibody recognizes it, such as by binding to it.

The term “ortholog” as used herein refers to a polynucleotide from one species that corresponds to a polynucleotide in another species; the two polynucleotides are related through a common ancestral species (a homologous polynucleotide). However, the polynucleotide from one species has evolved to become different from the polynucleotide of the other species.

The term “vaccine” as used herein refers to a composition that provides immunity to an individual upon challenge.

The term “subunit vaccine” as used herein refers to a vaccine wherein a polypeptide or fragment thereof is employed, as opposed to an entire organism.

A number of embodiments of the invention have been described. Nevertheless, it will be understood that various modifications may be made without departing from the spirit and scope of the invention. Accordingly, other embodiments are within the scope of the following claims.

EXAMPLES Example 1: ECH1038 (EtpE) is Highly Expressed by E. chaffeensis in Mammalian Cells

Materials and Methods E. chaffeensis and host cell culture. E. chaffeensis Arkansas type strain was propagated in DH82 cells, and host cell-free E. chaffeensis was obtained by controlled sonication as described [Rikihisa Y, et al. (1994) J Clin Microbiol 32: 2107-2112; Barnewall R E, et al. (1994) Infect Immun 62: 4804-4810]. Human peripheral blood monocytes were derived from buffy coats; HEK293, RF/6A and THP-1 cells were cultured as previously described [Liu H, et al. (2012) Cell Microbiol 14: 1037-1050; Miura K, et al. (2011) Infect Immun 79: 4947-4956; Barnewall R E, et al. (1994) Infect Immun 62: 4804-4810]. BMDMs were established from wild-type and DNase X ^(-/-) mice as described [Miura K, et al. (2011) Infect Immun 79: 4947-4956].

Production of recombinant proteins rEtpE-N and rEtpE-C, and antisera against them. DNA fragments encoding EtpE-C and EtpE-N were amplified by PCR with Phusion high-fidelity DNA polymerase (NEB) using E. chaffeensis chromosomal DNA as template. The fragments were cloned into pET33b(+) vector (Novagen); recombinant proteins were expressed in E. coli BL21 (DE3) and purified by Ni-affinity chromatography. The antibody against rEtpE-C was produced in ICR mice (Harlan), and the antibody against rEtpE-N was produced in rabbits.

Statistical analysis. Statistical analysis was performed by unpaired two-tailed Student's t-test. P<0.05 was considered to be significant.

Results

ECH1038 (GenBank accession no. YP_507823, EtpE) consists of 1963 amino acid residues (M_(r) 222,638, pI: 7.0) and is predicted to be an outer membrane protein with an N-terminal secretion signal by PSORT analysis [Miura K, Rikihisa Y (2007) Infect Immun 75: 3604-3613]. Although EtpE is variable in the central approximately 950 residues, the N-terminal approximately 700 residues and C-terminal approximately 300 residues are conserved among multiple E. chaffeensis strains of distinct virulence, suggesting that these two regions are indispensable for E. chaffeensis. The amino acid sequence of EtpE orthologs in the three strains of E. chaffeensis, Arkansas, Wakulla, and Liberty are provided in SEQ ID NO:1 (YP_507823), SEQ ID NO:10 (Accession No. DQ924562), and SEQ ID NO:11 (Accession No. DQ924563), respectively. Amino acid sequence alignment of EtpE orthologs among three genome-sequenced Ehrlichia species, E. chaffeensis Arkansas, E. canis Jake and E. ruminantium Welgevonden, revealed that while most of the N-terminal proximal region was conserved also among Ehrlichia species, the C-terminal region was not.

To begin probing EtpE function, N-terminal (residues 29-708) and C-terminal (residues 1656-1963) of EtpE were cloned as C-terminal histidine-tagged fusion proteins (rEtpE-N and rEtpE-C) and antisera were prepared against rEtpE-N and rEtpE-C. Western blot analysis using these antibodies showed that full-length EtpE was expressed by E. chaffeensis in DH82 cells (FIG. 1A). DH82 cells were initially used, since this cell line has been successfully used to culture isolate E. chaffeensis from the blood of HME patients [Dawson J E, et al. (1991) J Clin Microbiol 29: 2741-2745; Paddock C D, et al. (1997) J Clin Microbiol 35: 2496-2502].

To determine whether EtpE is expressed by E. chaffeensis in human monocytes, the pathogen's primary in vivo target cells, EtpE expression was determined in E. chaffeensis cultured in human primary macrophages derived from peripheral blood monocytes by double immunofluorescence labeling after paraformaldehyde (PFA) fixation and saponin permeabilization. E. chaffeensis major outer membrane protein P28 [Ohashi N, et al. (1998) Infect Immun 66: 132-139] was used as positive control to label the bacterial membrane. The results showed that EtpE was abundantly expressed by E. chaffeensis in human macrophages, and localized at bacterial membrane like P28 [Ohashi N, et al. (1998) Infect Immun 66: 132-139] (FIG. 1B).

Example 2: EtpE is Exposed on the E. chaffeensis Surface, and anti-EtpE-C Inhibits E. chaffeensis Binding, Entry, and Infection

Materials and Methods

Binding and internalization assay of E. chaffeensis and immunostaining of host cell-free E. chaffeensis. Coverslip cultures of DH82, HEK293, RF/6A cells, or macrophages differentiated from human peripheral blood monocytes or established from bone-marrow of DNase X^(-/-) or congenic wild-type mice and suspension culture of THP-1 cells were incubated with E. chaffeensis freshly isolated from infected cells at approximate multiplicity of infection (MOI) of 200, unless otherwise noted, for 30 to 45 min for binding assays or 2 to 4 h for internalization assays at 37° C. in 5% CO²/95% air. Cells were washed with phosphate-buffered saline (PBS: 137 mM NaCl, 2.7 mM KC1, 8.1 mM Na₂HPO₄, 1 mM KH₂PO₄, pH 7.4) to remove unbound bacteria and labeled with antibodies as described [Wang X, et al. (2006) Infect Immun 74: 1873-1882]. For binding assay cells were fixed with 3% PFA and labeled with mouse monoclonal anti-DNase X (Abcam), rabbit anti-E. chaffeensis P28 [Ohashi N, et al. (1998) Infect Immun 66: 132-139], mouse anti-rEtpE-C, or dog anti-E. chaffeensis [Barnewall R E, et al. (1997) Infect Immun 65:1455-1461] as primary antibodies and Alexa Fluor (AF) 488-conjugated goat anti-mouse IgG, AF555-conjugated goat anti-rabbit IgG (Invitrogen), or Texas Red-conjugated goat anti-dog IgG (Jackson ImmunoLab) as secondary antibodies. For internalization assays, two steps of labeling of fixed cells with anti-P28 were carried out as described: the first labeling step was performed without saponin permeabilization using AF488-conjugated goat anti-rabbit IgG, and the second labeling was performed with permeabilization using AF555-conjugated goat anti-rabbit IgG [Niu H, et al. (2006) Cell Microbiol 8: 523-534]. Fluorescent images were acquired using a Nikon Eclipse E400 fluorescence microscope with a xenon-mercury light source (Nikon), Deltavision deconvolution microscope (Applied Precision) with 0.2 or 0.4-μm step size along the z-axis of the cells, or an LSM 510 laser-scanning confocal microscope (Carl Zeiss). For immunostaining of live bacteria, host cell-free E. chaffeensis was incubated with anti-EtpE-C, anti-EtpE-N or E. chaffeensis P28 for 1 h at room temperature followed by fixing with 3% PFA and labeling with AF555-conjugated goat anti-mouse or anti-rabbit antibodies. To further demonstrate the surface exposure of EtpE, host cell-free E. chaffeensis was incubated with either pronase E (Sigma) at a concentration of 2 mg/ml in PBS or vehicle control for 15 min at 37° C. [Yoshiie K, et al. (2000) Infect Immun 68: 1125-1133]; pronase E was inactivated by adding 10% fetal bovine serum (FBS), followed by washing in PBS twice. The bacteria were cytospun onto glass slides, fixed with 3% PFA, followed by quenching in PBS containing 0.1 M glycine, washed with PBS and labeled sequentially with anti-EtpE-C and anti-CtrA [Cheng Z, et al. (2011) Mol Microbiol 82: 1217-1234] with or without saponin permeabilization followed by AF488 or AF555-conjugated goat anti-mouse or anti-rabbit antibodies.

[³⁵S]methionine-labeled E. chaffeensis binding and uptake. Approximately 10⁶ cells of E. chaffeensis-infected THP-1 cells/ml in 2 ml of methionine cysteine-deficient RPMI 1640 medium (ICN Biomedicals) supplemented with 10% FBS and 2 mM L-Gln were incubated with cycloheximide (Sigma) at 10 μg/ml at 37° C. for 1 h. A metabolic labeling reagent (Tran³⁵S-Label; 11.7 mCi/ml [1,100 Ci/mmol]; 100 μl; ICN Biomedicals) was added and the mixture was incubated further at 37° C. for 24 h. The radiolabeled E. chaffeensis was released by sonication and washed by centrifugation at 10,000 xg for 10 min. To study the effect of rabbit anti-P28 on E. chaffeensis binding and entry, radiolabeled E. chaffeensis cells (40,000 cpm/200 μl) preincubated with Fab fragment of anti-P28 IgG [0.5 mg/ml, prepared using Immobilized papain (Pierce) from IgG affinity purified with AffiPack Immobilized Protein A column (Pierce)] or Fab fragment of normal rabbit IgG (0.5 mg/ml) were added to 1×10⁶ THP-1 cells in 0.4 ml of RPMI 1640 medium containing 10% FBS and 2 mM L-Gln and incubated at 4° C. for 2 h. The uptake of E. chaffeensis was evaluated following removal of bound E. chaffeensis cells by incubation with pronase E at 2 mg/ml in PBS at 37° C. for 10 min after incubation of E. chaffeensis with THP-1 cells at 37° C. for 3 h. THP-1 cells were washed by centrifugation at 375 xg for 5 min, the cells then were dissolved in 0.6 N NaOH and 0.5% SDS, and the radioactivity was measured in a scintillation counter.

Results

P28 is bacterial surface exposed [Ohashi N, et al. (1998) Infect Immun 66: 132-139] and is a β-barrel protein that functions as porin [Kumagai Y, et al. (2008) J Bacteriol 190: 3597-3605]. To determine whether EtpE is exposed on the bacterial surface, double immunofluorescence labeling with anti-EtpE-C and anti-P28 was performed after PFA fixation without saponin permeabilization using E. chaffeensis bound to the surface of DH82 cells. Unlike methanol or acetone fixation, PFA fixation does not allow antibody penetration across biological membranes unless with subsequent permeabilization, thereby limiting antibody staining to molecules exposed to the cell surface [Wang X, et al. (2006) Infect Immun 74: 1873-1882]. The result showed labeling of both EtpE and P28 (FIG. 1C). Of note, labeled EtpE on E. chaffeensis had a beaded (rosary-like) pattern encircling individual bacterium, in contrast to P28 that had a uniform ring pattern (FIG. 1C). When host cell-free bacteria were treated with pronase E, the surface immunofluorescence staining of EtpE was abolished, but not of CtrA which is an E. chaffeensis cytosolic response regulator of a two-component system [Cheng Z, et al. (2011) Mol Microbiol 82: 1217-1234] (FIG. 9). These data indicate the surface exposure of EtpE. In contrast to the punctate labeling pattern of EtpE in host cell-bound bacteria, homogeneous labeling of EtpE was observed on host cell-free bacteria (FIG. 9).

Given the surface exposure of EtpE on E. chaffeensis, experiments were conducted to determine whether the antibody against EtpE inhibits binding, entry, and infection of E. chaffeensis. Among the several host cell types used in this study, primary monocytes, macrophages, and myelocytic leukemia cell lines (DH82 and THP-1 cells) are referred to as phagocytes. Phagocytes are very efficient in bacteria and particle uptake as they have an array of dedicated phagocytic receptors, including pathogen pattern recognition receptors, mannose receptors, scavenger receptors, receptors for immunoglobulin (FcR) and complement (CR3) that utilize opsonins for ingestion, to name a few [Krieger M (1997) Curr Opin Lipidol 8: 275-280; Aderem A, et al. (1999) Annu Rev Immunol 17: 593-623]. The other two cell lines used in this study, RF/6A endothelial and HEK293 epithelial cells, are referred to as non-phagocytes, since they lack these features. Non-phagocytes were first used to study the effect of in vitro antibody neutralization of EtpE as they lack the response to opsonization and will not readily take-up opsonized particles. E. chaffeensis was pre-incubated with mouse anti-EtpE-C or preimmune mouse sera, and then incubated with RF/6A cells. Binding and entry were determined by immunofluorescence labeling of E. chaffeensis with anti-P28 at 30 min and 2 h post-incubation/infection (pi), respectively. Infection was determined at 48 h pi by quantitative realtime PCR (qPCR). Anti-EtpE-C blocked E. chaffeensis binding, entry, and subsequently infection by approximately 80% compared to preimmune serum (FIG. 1D-1F). Similar level of inhibition of binding and entry was observed using mouse anti-EtpE-C in phagocytic cells such as human THP-1 cells (FIGS. 10A and 10B) and canine DH82 cells. This suggests that human or canine FcR-mediated entry of E. chaffeensis opsonized with mouse anti-EtpE-C was negligible in this experiment. Immunization of mice with recombinant P28, which functions as a porin [Kumagai Y, et al. (2008) J Bacteriol 190: 3597-3605], protects mice from E. chaffeensis challenge [Ohashi N, et al. (1998) Infect Immun 66: 132-139]. Additionally, in a mouse model of HME, immunization of mice with Ehrlichia muris P28 conferred protection from E. muris challenge [Crocquet-Valdes P A, et al. (2011) Clin Vaccine Immunol 18: 2018-2025]. As another control, to rule out the possibility that inhibition of binding is a general property of antibody neutralization of any E. chaffeensis cell surface proteins, experiments were conducted to determine whether antibody against P28 blocks E. chaffeensis binding and entry. The result showed antibody (Fab fragment) against P28 did not block binding or entry of E. chaffeensis (FIG. 11A and 11B). Taken together, these results suggest that EtpE-C potentially serves as an invasin to trigger E. chaffeensis entry in both phagocytes and non-phagocytes.

EtpE is predicted to be anchored on the bacterial outer membrane at its N-terminus, based on analysis using the PREDTMBB webserver [Miura K, Rikihisa Y (2007) Infect Immun 75: 3604-3613; Bagos P G, et al. (2004) Nucleic Acids Res 32: W400-404]. In contrast to anti-EtpE-C, anti-EtpE-N-pretreatment reduced E. chaffeensis infection by only 20% (FIG. 12A). Since both anti-EtpE-N and anti-EtpE-C reacted with native EtpE protein from E. chaffeensis equally well by Western blot analysis, accessibility of anti-EtpE-N to EtpE molecules was tested on live E. chaffeensis surface. For this purpose, the host cell-free E. chaffeensis was freshly prepared and incubated with the antibodies without pre-fixation. The result showed that E. chaffeensis was not as readily labeled with anti-EtpE-N as with anti-EtpE-C (FIG. 12B), suggesting that the antibody access to the N-terminal conserved region might be limited in the native conformation of EtpE in live E. chaffeensis.

Example 3: EtpE is Expressed in HME Patients and Infected Dogs, and Immunization with rEtpE-C Suppresses E. chaffeensis Infection in Mice

Materials and Methods

Western blot analysis with sera from HME patients and E. chaffeensis-infected dogs. Affinity-purified rEtpE-C and rEtpE-N (5 μg each) were subjected to SDS-PAGE, transferred to a nitrocellulose membrane, and incubated with sera from E. chaffeensis-infected dogs (CTUALJ, 3918815, 1425) [Huang H, et al. (2008) Infect Immun 76: 3405-3414], HME patients (ID: MRL1-22, MRL1-40, 72088) [Unver A, et al. (1999) J Clin Microbiol 37: 3888-3895], or control sera. After washing, the membranes were incubated with horseradish peroxidase-conjugated goat anti-dog or anti-human IgG (KPL). Reacting bands were visualized with enhanced chemiluminescence (ECL), images were captured and densitometric analysis was performed using an LAS3000 image documentation system (FUJIFILM Medical Systems).

Mouse infection studies. Two groups of C3H/HeJ mice (4-week-old females; 4 mice per group) (Jackson Laboratories) received either minced SDS-polyacrylamide gel containing 50 μg of rEtpE-C or minced gel alone, with Quil A (Accurate Chemicals) as adjuvant for a total of three times at 14-day intervals. E. chaffeensis challenge was performed 10 days following the last immunization as described [Ohashi N, et al. (1998) Infect Immun 66: 132-139]. DNase X^(-/-) [Rashedi I (2008) The Role of DNase X in Skeletal Muscle Addressed by Targeted Disruption of the Gene in a Mouse Model. Winnipeg: University of Manitoba. 122] and congenic wild-type C57BL/6 mice (5-to 6-week-old females; 5 mice per group) were inoculated intraperitoneally with E. chaffeensis-infected THP-1 cells (>90% cells infected; 6×10⁵ cells/mouse). DNA was extracted from blood samples using a QIAamp blood kit (Qiagen), and subjected to qPCR using E. chaffeensis 16S rDNA and mouse glyceraldehyde 3-phosphate dehydrogenase (G3PDH) gene primers.

Results

Because EtpE is highly expressed by E. chaffeensis in mammalian cells in vitro, experiments were conducted to determine whether EtpE is expressed in vivo by Western blot analysis of defined HME patient sera [Unver A, et al. (1999) J Clin Microbiol 37: 3888-3895]. Equal quantities of rEtpE-N and rEtpE-C (GelCode Blue staining shown in FIG. 2A) were used as antigens in the assay. Patient sera recognized both rEtpE-N and rEtpE-C, whereas the control serum from a healthy individual in an HME non-endemic region did not react with the recombinant proteins (FIG. 2B). Similarly, sera from dogs experimentally infected with E. chaffeensis [Huang H, et al. (2008) Infect Immun 76: 3405-3414], that were previously shown to recognize E. chaffeensis OmpA [Cheng Z, et al. (2011) Mol Microbiol 82: 1217-1234] and other E. chaffeensis lipoproteins [Huang H, et al. (2008) Infect Immun 76: 3405-3414], recognized both rEtpE-N and rEtpE-C, but the control dog serum did not (FIG. 2B). These data indicated that EtpE is expressed by E. chaffeensis in vivo during infection of its natural hosts, humans and dogs, and that an antibody (humoral) response is mounted against this protein during infection and disease.

Antibodies contribute to immunity against E. chaffeensis in immunocompetent mice [Yager E, et al. (2005) Infect Immun 73: 8009-8016]. Given the facts that anti-EtpE-C neutralized E. chaffeensis binding, consequently entry and infection in vitro, EtpE was expressed by E. chaffeensis in vivo and that a humoral immune response was mounted in infected mammals, experiments were conducted to examine whether rEtpE-C immunization could confer protection in mice from E. chaffeensis challenge. C3H/HeJ strain of mice was used, since this strain was reported to serve as a useful model for studying E. chaffeensis infection [Telford SR (1996) Vet Microbiol 52: 103-112]. At 10 days after the last immunization, all mice were challenged intraperitoneally with E. chaffeensis. The E. chaffeensis load in the blood from rEtpE-C-immunized mice at 5 days post challenge was significantly lower than that of nonimmunized mice (FIG. 2C). These results indicate that rEtpE-C is a protective immunogen relevant in E. chaffeensis infection in vivo.

Example 4: Entry of rEtpE-C-Coated Beads into Macrophages is Blocked by Compounds that Block E. chaffeensis Invasion

Materials and Methods

Binding and internalization of latex beads. Sulfate-modified fluorescent red polystyrene beads (0.5 μm diameter; Sigma) at 3-4×10⁶ beads in 200 μl of 25 mM 2-(N-morpholino)ethanesulfonic acid (MES) buffer, pH 8.0 were incubated with 1 mg of rEtpE-C or rEtpE-N proteins in 5-7 μl 7 M urea in 50 mM sodium phosphate buffer, pH 7.2 at 4° C. overnight with mixing at 20 rpm. MES buffer (150 ml) was sequentially added to the mixture every 15 min and incubated at room temperature, rotating at 20 rpm eventually diluting to around 200 times the original volume of urea buffer. rECH0825 and rGroEL were treated similarly, but without urea. The coated beads were collected by low speed centrifugation, washed twice in MES buffer and re-suspended in complete DMEM or advanced MEM media, then gently sonicated to disperse the beads. Protein coating of the beads were confirmed by dot blot assay and/or immunofluorescence labeling. Freshly prepared protein-coated or non-coated beads were added at a multiplicity of approximately 50 beads per cell for co-localization studies and 500 beads per cell for quantitation of binding and internalization studies. The beads were incubated with HEK293 or RF/6A cells for 1 h at 37° C. Unbound beads were removed by washing and cells were fixed for immunofluorescence labeling to detect the localization of DNase X or EEA1 (anti-EEA1, BD). To study the effect of MDC, genistein, or verapamil on bead internalization, RF/6A cells were incubated with these chemicals at a final concentration of 100 mM or 0.1% DMSO solvent control for 30 min, then with rEtpE-C-coated beads for 8 h at 37° C. BMDMs from wild-type mice were pre-incubated with MDC or genistein (100 mM), PI-PLC (5 U/ml) or 0.1% DMSO for 30 min and then incubated with rEtpE-C-coated or non-coated beads for 45 min at 37° C. PI-PLC-treated cells were washed prior to addition of rEtpE-C-coated beads. The cells were washed and treated with 0.25% trypsin at 37° C. for 10 min to remove surface-bound beads. The detached cells were further washed by low-speed centrifugation and later cytocentrifuged onto a glass slide and fixed with 3% PFA to observe internalized beads. To estimate the number of bound beads, a similar procedure for observing internalized beads was followed except that the beads were incubated with BMDM for 30 min at 4° C. and following incubation the cells were washed to remove loosely bound beads and directly fixed with 3% PFA without trypsin treatment. For scanning electron microscopy, rEtpE-C-coated beads were incubated with RF/6A cells for 2 h at 37° C. and processed as described previously [Thomas S, et al. (2010) PLoS One 5: e157751]. For transmission electron microscopy, coated beads were incubated with RF/6A cells for 8 h at 37° C. and processed as described previously [Rikihisa Y, et al. (1979) J Exp Med 150: 703-708]. The 3D orthogonal view of the cell to show spatial distribution of DNase X with beads was obtained by using the volume viewer function of SoftWoRx DeltaVision image acquisition software from Applied Precision.

Live-cell imaging. RF/6A cells were cultured in 35-mm glass bottom dishes (Wilco), transfected with DNase X-GFP, and incubated with rEtpE-C-coated beads at 4° C. for 1 h to facilitate bead binding, but prevent internalization. Unbound beads were washed off, cells were replenished with medium lacking phenol red, and the samples moved to a controlled environmental chamber at 37° C. with under 5% CO²/95% air. Time-lapse images were acquired at an interval of 10 s for 5 to 20 min through a 60×1.42 NA oil immersion lens with an inverted Olympus IX-70 microscope, in 0.4-μm steps in the z-axis using the attached Applied Precision motorized stage (DeltaVision deconvolution microscope). All stacks of images were deconvoluted using SoftWoRx software and the time-lapse images of a single focal plane of 0.4-μm focal depth at the cell surface were exported as a video.

Results

Bacterial surface exposure of EtpE-C and effectiveness of EtpE-C as the target for both in vitro and in vivo neutralization suggest that EtpE-C may mediate E. chaffeensis invasion. To investigate this possibility, fluorescent latex beads of average size of 0.5 μm (similar to the size of infectious DCs of E. chaffeensis) were coated with rEtpE-C protein. The presence of rEtpE-C on beads was confirmed by dot-blot analysis and immunofluorescence labeling with antiserum against EtpE-C (FIG. 3A). Beads were incubated with mouse bone marrow-derived macrophages (BMDMs) for 45 min followed by trypsin treatment to remove beads that were not internalized. Mouse BMDMs were used here, also to serve as the wild-type control for the later studies using BMDMs from mutant mice. rEtpE-C-coated beads entered BMDMs (FIGS. 3B and 3C). Treatment with MDC, genistein (broad-spectrum protein tyrosine kinase inhibitor), or phosphatidylinositol-specific phospholipase C (PI-PLC that removes GPI-anchored proteins from the cell surface) blocks E. chaffeensis entry and infection of THP-1 cells [Lin M, et al. (2002) Infect Immun 70: 889-898; Lin M, Rikihisa Y (2003) Cell Microbiol 5: 809-820]. The entry of rEtpE-C-coated beads into BMDMs was almost completely blocked by these treatments (FIGS. 3B and 3C), suggesting rEtpE-C-coated beads enter BMDMs by the same signaling pathway as E. chaffeensis does. The latex bead is well-known to be taken up by macrophages and has been used as a model to study phagocytosis [Werb Z, et al. (1972) J Biol Chem 247: 2439 -2446]. In striking contrast, entry of non-coated beads into BMDMs was not blocked by any of these treatments (FIG. 3D).

Example 5: rEtpE-C-Coated Beads Enter Non-Phagocytes

Results

Non-coated beads did not bind or enter RF/6A and HEK293 non-phagocytic cells (HEK293 cell data are shown in FIG. 4B). Remarkably, rEtpE-C-coated beads did readily bind and enter non-phagocytes (HEK293 data are shown in FIGS. 4A and 4B). Beads coated with other recombinant E. chaffeensis proteins including rEtpE-N, rECH0825 (a type IV secretion effector protein) [Liu H, et al. (2012) Cell Microbiol 14: 1037-1050] or rECH0365 (GroEL) did not bind HEK293 cells (FIGS. 4A and 4B), indicating binding and entry of beads into nonphagocytes was due to specific coating with EtpE-C. Scanning and transmission electron microscopy revealed that rEtpE-C-coated beads bound to RF/6A cells were associated with filopodia-like membrane projections (FIGS. 4C and 4D left panel) similar to those surrounding E. chaffeensis bound to DH82 cells [Zhang J Z, et al. (2007) Cell Microbiol 9: 610-618]. Transmission electron microscopy of RF/6A cells incubated with rEtpE-C-coated beads verified that the beads were indeed internalized into RF/6A cells (FIG. 4D right panel). MDC, genistein, and verapamil (a Ca²⁺channel blocker) that block E. chaffeensis entry into THP-1 cells [Lin M, et al. (2002) Infect Immun 70: 889-898], also blocked E. chaffeensis entry into RF/6A cells (FIG. 13). Treatment with any of these compounds almost completely blocked the entry of rEtpE-Ccoated beads into RF/6A cells (FIGS. 4E and 4F). Once internalized, E. chaffeensis-containing vacuoles acquire characteristics of early endosomes [Mott J, et al. (1999) Infect Immun 67: 1368-1378]. To determine whether rEtpE-C-coated beads were delivered to early endosomes, immunofluorescence labeling was used to visualize the spatial relationship of the early endosomal marker, EEA1 with the rEtpE-C-coated beads, and observed by deconvolution microscopy. Individual as well as multiple beads were seen encased by EEA1-labeled membranous compartment, suggesting that some beads were in endosomes (FIG. 4G). These results indicate that EtpE-C is an invasin, and even in the absence of any other E. chaffeensis factors, EtpE-C alone is sufficient to mediate the binding and entry of EtpE-C-coated beads into non-phagocytic cells.

Example 6: EtpE-C Binds DNase X

Materials and Methods

Yeast two-hybrid screening. Yeast two-hybrid screening was performed using Matchmaker Two-Hybrid System (Clontech) according to manufacturer's instructions. The bait plasmid pGBKT7-EtpE-C was constructed by the fusion of EtpE-C with the GAL4 DNA-binding domain in pGBKT7 (Clontech) by PCR. EtpE-C coding sequence was amplified using the forward primer 5′-AATCCATGGA ATTGTTGTCA TTAGTTGGTG GGCATCG-3′ (SEQ ID NO:12) and reverse primer 5′-TCGACGGATC CAATCCCCTT CCAGCATTAA TTTTATCAAA GG-3′ (SEQ ID NO:13), and the product was ligated into pGBKT7. pGBKT7-EtpE-C was transformed into Saccharomyces cerevisiae strain AH109 and selected by the ability to grow on SD agar plates lacking tryptophan. The expression of bait protein EtpE-C in yeast was examined by Western blotting. The human bone marrow MATCHMAKER cDNA library (Clontech) that was fused with GAL4-activating domain in pGADT7 was transformed in S. cerevisiae strain Y187 (Clontech). Library clones expressing interacting prey proteins were screened with yeast mating. Positive clones were selected by their ability to grow on SD quadruple drop-out (SD/QDO) plates lacking adenine, histidine, leucine, and tryptophan, and verified on SD/QDO plates containing X-gal. Positive clones were then isolated, and the prey plasmids were purified and sequenced after they were transformed into E. coli TOP10F9 competent cells (Invitrogen). The interaction was confirmed by re-shuttling the purified prey plasmid into S. cerevisiae AH109 transformed with bait plasmid and by nutritional selection in SD/QDO plates.

Far-Western blotting, protein affinity pull-down and coimmunoprecipitation. Far-Western blotting was performed using 5 μg of rEtpE-C and rECH0825 that were separated by SDS-PAGE, transferred to a nitrocellulose membrane and renatured with serial guanidinium-HC1 treatment followed by incubation with THP-1 cell lysate in NP-40 lysis buffer (150 mM NaCl, 50 mM Tris-HC1 pH 7.4, 1% w/v NP-40, supplemented with 1% protease inhibitor cocktail set III [Calbiochem]) as described [Bao W, et al. (2009) J Bacteriol 191: 278-286]. After stringent washing, the membrane was incubated with anti-DNase X and peroxidase-conjugated goat anti-mouse antibodies (KPL). The membrane was stripped with Restore Western Blot Stripping Buffer (Thermo scientific) and re-probed with peroxidase-conjugated anti-histidine antibody (Sigma). For protein pull-down, His-tagged rEtpE-C was bound to and renatured on the Ni-affinity matrix (Promega). THP-1 cell lysate in NP-40 lysis buffer was applied to the matrix and incubated for 8 h at 4° C. After washing off the unbound or non-specifically bound proteins from the matrix, rEtpE-C and bound protein complex were eluted with 250 mM imidazole. The eluate and the post-elution Ni-matrix were resuspended in 26 SDS-sample buffer and subjected to Western blotting with anti-DNase X antibody. For co-immunoprecipitation assay, THP-1 cells were incubated with E. chaffeensis for 30 min and lysed in NP-40 lysis buffer. The lysate was immunoprecipitated with anti-EtpEC (2 μg)-bound protein A agarose or control mouse IgG (2 μg)-bound agarose beads. The precipitate was re-suspended in 2x SDS-sample buffer and subjected to Western blotting with anti-DNase X antibody.

Results

Since EtpE-C could mediate binding and entry of EtpE-C-coated beads, Experiments were conducted to search for the potential host-cell receptor for EtpE-C.

EtpE-C was cloned into the yeast two-hybrid bait vector and a human bone marrow cDNA prey library was screened to identify interacting proteins. Of the 5 clones detected and sequenced, all of them encoded a protein, deoxyribonuclease 1-like 1 (DNase 1L1, DN1L1, or DNase X on chromosome Xq28, GenBank accession no: X90392, 302 residues). One of the clones contained an additional plasmid encoding

S-adenosyl methionine-dependent methyltransferase but the coding sequence was out-of-frame; this prey construct alone did not support yeast growth when co-transformed with bait vector to test their interaction. All sequence hits corresponded to the C-terminal fragment of DNase X (residues 105-302). DNase X, one of the human DNase I-family endonucleases, is expressed on the cell surface as a GPI-anchored protein and also localized at early endocytic vesicles, endoplasmic reticulum, and Golgi [Shiokawa D, et al. (2001) Biochemistry 40: 143-152; Shiokawa D, et al. (2007) J Biol Chem 282:17132-17140].

To confirm EtpE-C binding to the native human DNase X, far-Western blot analysis was performed. DNase X from the THP-1 cell lysate bound to re-natured rEtpE-C on a nitrocellulose membrane, whereas DNase X did not bind the control rECH0825 (FIG. 5A). Next, a protein pull-down assay was used wherein THP-1 cell lysate was applied to rEtpE-C bound to and renatured on a Ni-affinity matrix. Western blotting showed that native DNase X from the lysate bound to rEtpE-C, but not to the control rECH0825 (FIG. 5B). In addition, co-immunoprecipitation showed that anti-EtpE-C, but not the control mouse IgG pulled down native DNase X from the lysate of THP-1 cells incubated with E. chaffeensis for 30 min (FIG. 5C). Taken together, these results indicate that EtpE-C can bind to DNase X.

RF/6A or HEK293 cells incubated with rEtpE-C-coated beads were fixed, and without membrane permeabilization, immunofluorescence labeled cell surface-exposed DNase X was conducted. DNase X localized to the areas on the surface of cells where rEtpE-C-coated beads were present (RF/6A cell image shown in FIG. 5D). Timelapse live-cell image analysis of rEtpE-C-coated beads bound to RF/6A cells ectopically expressing DNase X-GFP at 4° C. showed that, upon warming up to 37° C., the initially separated DNase X-GFP signal and beads became closer and overlapped within 5 min (FIG. 5E). The fluorescence intensity profile analysis of red (rEtpE-C-coated beads) and green (DNase X-GFP) signal along the length of the line also revealed that the signals separated at initial time points converged in a few min after warming-up (FIG. 5F).

Example 7: Binding and Internalization of rEtpE-C-Coated Beads is Dependent on DNase X

Results

Since DNase X localized to EtpE-C-coated beads in nonphagocytes, this phenomenon was next examined in phagocytes. Human primary macrophages derived from peripheral blood monocytes were incubated with rEtpE-C-coated or non-coated beads, cell surface exposed DNase X was immunofluorescence-labeled without permeabilization and the distribution of beads and DNase X was examined by deconvolution microscopy. Surface DNase X was seen clustered with rEtpE-C-coated beads; whereas both surface DNase X and beads were randomly dispersed with non-coated beads (image in a single z-plane shown in FIG. 6A). Orthogonal views of the cell from the reconstructed 3D view of serial z-stack images unequivocally demonstrated colocalization of DNase X with rEtpE-C-coated beads (FIG. 6B left panel), whereas DNase X did not colocalize with non-coated beads (FIG. 6B right panel). The intensity profile analysis of green (DNase X) and red (beads) signals of a single optical section showed that DNase X coincided with rEtpE-C-coated beads, but not with noncoated beads (FIG. 6B right panels). Similar results were observed with canine primary macrophages derived from peripheral blood monocytes and DH82 cells (FIG. 14). These results indicate DNase X localizes to rEtpE-C-coated beads in primary human and canine macrophages, the pathogen's in vivo target cells.

rEtpE-C-coated beads entered wild-type mouse BMDMs as shown in FIGS. 3B and 3C. Therefore, experiments were conducted to determine whether rEtpE-C-coated beads can enter BMDMs from congenic DNase X^(-/-) mice. Beads were incubated with BMDMs from DNase X^(-/-) mice for 45 min followed by trypsin treatment to remove beads that were not internalized. Results showed rEtpE-C-coated beads did not enter

DNase X^(-/-) BMDMs (FIGS. 6C and 6D). In striking contrast, non-coated beads freely entered DNase X^(-/-) BMDMs (FIGS. 6C and 6D). This lack of entry of rEtpE-C-coated beads into DNase X^(-/-) BMDM, but not into the wild-type BMDM, was a direct consequence of its failure to bind DNase X^(-/-) BMDM (FIG. 15). This phenomenon was specific to rEtpE-C-coated beads, because neither the non-coated beads nor the rECH0825-coated beads showed any defect in binding DNase X^(-/-) BMDMs (FIG. 15). Taken together, these results indicate that rEtpE-C coating dictates the latex bead binding and entry via DNase X-dependent pathway.

Example 8: DNase X Mediates E. chaffeensis Binding, Entry, and Infection

Materials and Methods

In vitro neutralization and RNA interference. E. chaffeensis preincubated with 25 μg/ml of mouse anti-rEtpEC, rabbit anti-rEtpE-N, or preimmune mouse or rabbit sera for 1 h at 4° C. were used to infect THP-1, RF/6A, or DH82 cells. Alternatively, E. chaffeensis was added to DH82 cells preincubated with 10 μg/ml of monoclonal anti-DNase X or control mouse monoclonal antibody for 30 min at 25° C. in serum-free DMEM. Binding, internalization, and infection were determined at 30 min, 2 h and 48 h pi, respectively. HEK293 cells in 24-well plates were transfected with 50 nM DNase X siRNA (Santa Cruz Biotechnology) or scrambled control siRNA using Lipofectamine 2000 (Invitrogen). A second transfection with 50 nM of DNase X and scrambled siRNAs was performed 30 h after the first transfection. An aliquot of cells were harvested at 24 h after the second transfection to determine the protein amount of DNase X by Western blotting and densitometry analysis with anti-DNase X and rabbit anti-actin (Sigma). The other aliquot of cells were incubated with E. chaffeensis and incubated for an additional 48 h to evaluate infection. Infection was determined by qPCR of E. chaffeensis 16S rRNA gene relative to host cell G3PDH gene [Cheng Z, et al. (2011) Mol Microbiol 82: 1217-1234].

Results

Since DNase X was localized to EtpE-C-coated bead entry foci, experiments were conducted to determine whether DNase X localizes to the E. chaffeensis entry foci as well. Double immunofluorescence labeling of non-permeabilized DH82 cells and primary human macrophages derived from human peripheral blood monocytes showed surface DNase X colocalization with the bound E. chaffeensis (FIGS. 7A and 7B). DNase X also localized to the areas of E. chaffeensis binding on THP-1 cells. When DH82 cells were pre-incubated with monoclonal anti-DNase X IgG to block the surface-exposed DNase X, E. chaffeensis binding, entry, and overall infection were significantly reduced compared with the control mouse IgG-treated DH82 cells (FIGS. 7C-7E). Next, a small interfering RNA (siRNA) against DNase X was used to reduce the expression of endogenous DNase X in HEK293 cells (FIG. 7F). Suppression of DNase X expression significantly reduced E. chaffeensis infection in HEK293 cells (FIG. 7G). Moreover, E. chaffeensis binding and entry were reduced by 60% in DNase X BMDMs compared to the wild-type BMDMs (FIG. 7H). E. chaffeensis load at 56 h pi was significantly lower in DNase X BMDMs compared to the wild-type BMDMs (FIG. 7I). These results demonstrated that effective E. chaffeensis binding, entry, and infection depended on DNase X. Importantly, E. chaffeensis load in peripheral blood at 5 days pi in DNase X^(-/-) mice was significantly lower than in wild-type mice (FIG. 7J), indicating that effective in vivo infection of E. chaffeensis also requires involvement of DNase X.

Unless defined otherwise, all technical and scientific terms used herein have the same meanings as commonly understood by one of skill in the art to which the disclosed invention belongs. Publications cited herein and the materials for which they are cited are specifically incorporated by reference.

Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments of the invention described herein. Such equivalents are intended to be encompassed by the following claims. 

What is claimed is:
 1. A vaccine, comprising (a) one or more polypeptides comprising an amino acid sequence having at least 70% identity to an amino acid sequence selected from the group consisting of SEQ ID NO:1, SEQ ID NO:3, SEQ ID NO:5, or a an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp.; and (b) a pharmaceutically acceptable adjuvant.
 2. The vaccine of claim 1, wherein the one or more polypeptides comprise an amino acid sequence having at least 70% identity to SEQ ID NO:2 (residues 1656-1963 of SEQ ID NO:1), SEQ ID NO:4 (residues 1408-1510 of SEQ ID NO:3), SEQ ID NO:6 (residues 1410-1710 of SEQ ID NO:5), or a an immunogenic fragment thereof capable of eliciting an immune response against an Ehrlichia sp.
 3. The vaccine of claim 1, comprising at least two polypeptides collectively capable of eliciting an immune response against at least two Ehrlichia sp.
 4. The vaccine of claim 3, comprising at least three polypeptides collectively capable of eliciting an immune response against at least three Ehrlichia sp.
 5. The vaccine of any one of claims 1 to 4, wherein the vaccine is capable of eliciting an immune response against Ehrlichia chaffeensis.
 6. The vaccine of claim 5, wherein at least one of the one or more polypeptides comprise SEQ ID NO:1, SEQ ID NO:2, or an immunogenic fragment thereof capable of eliciting an immune response against Ehrlichia chaffeensis.
 7. The vaccine of claim 1, wherein the vaccine is capable of eliciting an immune response against Ehrlichia canis.
 8. The vaccine of claim 7, wherein at least one of the one or more polypeptides comprise SEQ ID NO:3, or an immunogenic fragment thereof capable of eliciting an immune response against Ehrlichia canis.
 9. The vaccine of any one of claims 1 to 8, wherein the vaccine is capable of eliciting an immune response against Ehrlichia ruminantium.
 10. The vaccine of claim 9, wherein at least one of the one or more polypeptides comprise SEQ ID NO: 5, or an immunogenic fragment thereof capable of eliciting an immune response against Ehrlichia ruminantium.
 11. The vaccine of claim 1, wherein the vaccine is capable of eliciting an immune response against Ehrlichia muris, Ehrlichia ewingii, or a combination thereof.
 12. The vaccine of claim 1, wherein the adjuvant is selected from the group consisting of Quil A, aluminum salts, squalene, virosomes, and combinations thereof.
 13. The vaccine of claim 1, wherein the immune stimulant comprises cytokines, growth factors, chemokines 